US20110120871A1 - Formation of Layers of Amphiphilic Molecules - Google Patents
Formation of Layers of Amphiphilic Molecules Download PDFInfo
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- US20110120871A1 US20110120871A1 US12/809,327 US80932708A US2011120871A1 US 20110120871 A1 US20110120871 A1 US 20110120871A1 US 80932708 A US80932708 A US 80932708A US 2011120871 A1 US2011120871 A1 US 2011120871A1
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- B01L3/502707—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by the manufacture of the container or its components
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- B01L3/50273—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip characterised by the means or forces applied to move the fluids
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- G01N27/28—Electrolytic cell components
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- G01N27/327—Biochemical electrodes, e.g. electrical or mechanical details for in vitro measurements
- G01N27/3275—Sensing specific biomolecules, e.g. nucleic acid strands, based on an electrode surface reaction
- G01N27/3278—Sensing specific biomolecules, e.g. nucleic acid strands, based on an electrode surface reaction involving nanosized elements, e.g. nanogaps or nanoparticles
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- G01N27/26—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means by investigating electrochemical variables; by using electrolysis or electrophoresis
- G01N27/416—Systems
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- G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
- G01N33/483—Physical analysis of biological material
- G01N33/487—Physical analysis of biological material of liquid biological material
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- G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
- G01N33/483—Physical analysis of biological material
- G01N33/487—Physical analysis of biological material of liquid biological material
- G01N33/48707—Physical analysis of biological material of liquid biological material by electrical means
- G01N33/48721—Investigating individual macromolecules, e.g. by translocation through nanopores
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- B01L2300/06—Auxiliary integrated devices, integrated components
- B01L2300/0627—Sensor or part of a sensor is integrated
- B01L2300/0645—Electrodes
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- B01L2300/161—Control and use of surface tension forces, e.g. hydrophobic, hydrophilic
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- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0403—Moving fluids with specific forces or mechanical means specific forces
- B01L2400/0415—Moving fluids with specific forces or mechanical means specific forces electrical forces, e.g. electrokinetic
- B01L2400/0421—Moving fluids with specific forces or mechanical means specific forces electrical forces, e.g. electrokinetic electrophoretic flow
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- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0403—Moving fluids with specific forces or mechanical means specific forces
- B01L2400/0415—Moving fluids with specific forces or mechanical means specific forces electrical forces, e.g. electrokinetic
- B01L2400/0427—Electrowetting
Definitions
- the present invention relates to the formation of layers of amphiphilic molecules such as lipid bilayers. It is particularly concerned with the formation of high quality layers suitable for applications requiring measurement of electrical signals with a high degree of sensitivity, for example single channel recordings and stochastic sensing for biosensor or drug screening applications. In one particular aspect, it is concerned with applications employing arrays of layers of amphiphilic molecules, for example lipid bilayers. In another aspect, the present invention relates to the performance of an electrode provided in a recess, for example for conducting electro-physiological measurements.
- a layer of amphiphilic molecules may be used as the layer separating two volumes of aqueous solution.
- the layer resists the flow of current between the volumes.
- a membrane protein is inserted into the layer to selectively allow the passage of ions across the layer, which is recorded as an electrical signal detected by electrodes in the two volumes of aqueous solution.
- the presence of a target analyte modulates the flow of ions and is detected by observing the resultant variations in the electrical signal.
- Such techniques therefore allow the layer to be used as a biosensor to detect the analyte.
- the layer is an essential component of the single molecule biosensor presented and its purpose is two-fold. Firstly the layer provides a platform for the protein which acts as a sensing element. Secondly the layer isolates the flow of ions between the volumes, the electrical resistance of the layer ensuring that the dominant contribution of ionic flow in the system is through the membrane protein of interest, with negligible flow through the bilayer, thus allowing detection of single protein channels.
- a specific application is stochastic sensing, where the number of membrane proteins is kept small, typically between 1 and 100, so that the behaviour of a single protein molecule can be monitored.
- This method gives information on each specific molecular interaction and hence gives richer information than a bulk measurement.
- requirements of this approach are a very high resistance seal, typically at least 1 G ⁇ and for some applications one or two orders of magnitude higher, and sufficient electrical sensitivity to measure the currents.
- the requirements for stochastic sensing have been met in the laboratory, the conditions and expertise required limit its use.
- the laboratory methods are laborious and time-consuming and are not easily scalable to high-density arrays, which are desirable for any commercial biosensor.
- the fragility of single bilayer membranes means that anti-vibration tables are often employed in the laboratory.
- planar artificial lipid bilayers are known in the art, most notably including folded bilayer formation (e.g. Montal & Mueller method), tip-dipping, painting, patch clamping, and water-in-oil droplet interfaces.
- the method of Montal & Mueller (Proc. Natl. Acad. Sci. USA. (1972), 69, 3561-3566) is popular as a cost-effective and relatively straightforward method of forming good quality folded lipid bilayers suitable for protein pore insertion, in which a lipid monolayer is carried on the water/air interface past either side of an aperture in a membrane which is perpendicular to that interface.
- the lipid is added to the surface of the aqueous electrolyte solution by first dissolving it in an organic solvent, a drop of which is then allowed to evaporate on the surface of the aqueous solution on either side of the aperture.
- the solution/air interfaces are physically moved up and down past either side of the aperture until a bilayer is formed.
- the technique requires the presence of a hydrophobic oil applied as a pre-treatment coating to the aperture surface.
- the primary function of the hydrophobic oil is to form an annulus region between the bilayer and the aperture film where the lipid monolayers must come together over a distance typically between 1 and 25 ⁇ m.
- Tip-dipping bilayer formation entails touching the aperture surface (e.g. a pipette tip) onto the surface of a test solution that is carrying a monolayer of lipid. Again the lipid monolayer is first generated at the solution/air interface by evaporating a drop of lipid dissolved in organic solvent applied to the solution surface. The bilayer is then formed by mechanical actuation to move the aperture into/out of the solution surface.
- the aperture surface e.g. a pipette tip
- the drop of lipid dissolved in organic solvent is applied directly to the aperture, which is submerged in the aqueous test solution.
- the lipid solution is spread thinly over the aperture using a paint brush or equivalent. Thinning of the solvent results in formation of a lipid bilayer, however, complete removal of the solvent from the bilayer is difficult and consequently the bilayer formed is less stable and more noise prone during measurement.
- Patch-clamping is commonly used in the study of biological cell membranes, whereby the cell membrane is clamped to the end of a pipette by suction and a patch of the membrane becomes attached over the aperture.
- the method has been adapted for artificial bilayer studies by clamping liposomes which then burst to leave a lipid bilayer sealing over the aperture of the pipette. This requires stable giant unilamellar liposomes and the fabrication of small apertures in glass surfaced materials.
- Water-in-oil droplet interfaces are a more recent invention in which two aqueous samples are submerged in a reservoir of hydrocarbon oil containing lipid.
- the lipid accumulates in a monolayer at the oil/water interface such that when the two samples are brought into contact a bilayer is formed at the interface between them.
- the protein is then introduced to the bilayer either by random collision from the aqueous solution, by fusion of vesicles containing the protein, or by mechanically transporting it to the bilayer, for example on the end of a probe device such as an agar tipped rod.
- a large proportion of the devices that are capable of performing stochastic sensing form a bilayer by using a variant of the folded lipid bilayers technique or the painted bilayer technique. To date most have concentrated either on novel methods of aperture formation or on utilising the emerging technologies in micro fabrication to miniaturise the device or to create a plurality of addressable sensors.
- the devices of both Sandison et al. and Suzuki et al. are both miniaturised versions of a standard painted bilayer technique with two distinct fluidic chambers separated by a septum containing an aperture across which the bilayer is formed, one chamber being filled before the other.
- Sandison et al. created a device with three fluid chambers, each with separate fluidics, an approach which would be difficult to scale to large numbers of bilayers. Suzuki et al.
- biosensor device using a supported lipid bilayer is disclosed in U.S. Pat. No. 5,234,566.
- the device is capacitive.
- a gated ion channel responds to an analyte, the binding of this analyte causes a change in the gating behaviour of the ion channel, and this is measured via the electrical response of the membrane capacitance.
- To support the lipid bilayer there is used a monolayer of alkane-thiol molecules on a gold electrode, which provides a scaffold for a lipid monolayer to self-assemble onto.
- This monolayer can incorporate ion channels such as gramicidin which are used as the sensing element of the device.
- the first problem lies with the resistance of the bilayer membrane which is typically about 100 M ⁇ . While this may be suitable for examining protein behaviour at large protein concentrations, it is not sufficient for a high-fidelity assay based on single molecule sensing, typically requiring a resistance of at least 1 G ⁇ and for some applications one or two orders of magnitude higher.
- the second problem is the small volume of solution trapped in the short distance between the bilayer and the solid support, typically of the order of 1 nm. This small volume does not contain many ions, affecting the stability of the potential across the bilayer and limiting the duration of the recording.
- a number of methods have been proposed to overcome the problems with solid supported bilayers.
- One option is to incorporate a chemical linkage between the bilayer and the surface, either a small polyethylene glycol layer is introduced (polymer cushioned bilayers), or the lipid is chemically modified to contain a small hydrophilic linkage and reacted with the surface providing a scaffold for vesicle deposition (tethered bilayers). While these methods have increased the ionic reservoir beneath the lipid bilayer, they are inconvenient to implement and have done little to decrease the current leakage across the bilayer.
- a method of forming a layer separating two volumes of aqueous solution comprising:
- Such a method allows the formation of layers of amphiphilic molecules which are of sufficiently high quality for sensitive techniques such as stochastic sensing whilst using apparatus and techniques which are straightforward to implement.
- the apparatus used is relatively simple, involving most importantly a body of ionically non-conductive material having formed therein at least one recess. It has been demonstrated, surprisingly, that it is possible to form a layer of the amphiphilic molecules across such a recess simply by flowing the aqueous solution across the body to cover the recess.
- a pre-treatment coating of a hydrophobic fluid is applied to the body across the recess.
- the pre-treatment coating assists formation of the layer.
- the layer is formed without any need for a complicated apparatus involving two chambers separated by a septum and requiring a complicated fluidics arrangement to achieve separate filling. This is because the method does not require the recess to be pre-filled prior to introducing aqueous solution into the chamber above. Instead, the aqueous solution is introduced into the recess from the chamber. Despite this, it is still possible to form the layer by mere control of the aqueous solution flowing into the chamber. Such flow control is a straightforward practical technique.
- the method allows the formation of layers of amphiphilic molecules which are suitable for high sensitivity biosensor applications such as stochastic sensing and single channel recording. It has been demonstrated possible to form layers of high resistance providing highly resistive electrical seals, having an electrical resistance of 1 G ⁇ or more, typically at least 100 G ⁇ . which, for example, enable high-fidelity stochastic recordings from single protein pores. This is achieved whilst trapping a volume of aqueous solution in the recess between the layer and the electrode. This maintains a significant supply of electrolyte. For example, the volume of aqueous solution is sufficient to allow stable continuous dc current measurement through membrane proteins inserted in the layer. This contrasts significantly with the known techniques described above using supported lipid bilayers.
- the simple construction of the apparatus allows the formation of a miniaturised apparatus having an array of plural recesses and allowing the layer across each recess to be electrically isolated and individually addressed using its own electrode, such that the miniaturised array is equivalent to many individual sensors measuring in parallel from a test sample.
- the recesses may be relatively densely packed, allowing a large number of layers to be used for a given volume of test sample.
- Individual addressing may be achieved by providing separate contacts to each electrode which is simple using modern microfabrication techniques, for example lithography.
- the method allows the formation of multiple layers of the amphiphilic molecules within a single apparatus across the plural recesses in an array using a very straightforward technique.
- membrane proteins In most applications, one or more membrane proteins is subsequently inserted into the layer. Certain membrane proteins that can be used in accordance with the invention are discussed in more detail below.
- an apparatus suitable for implementing such methods of formation of a layer of amphiphilic molecules.
- the amphiphilic molecules are typically a lipid.
- the layer is a bilayer formed from two opposing monolayers of lipid.
- the lipids can comprise one or more lipids.
- the lipid bilayer can also contain additives that affect the properties of the bilayer. Certain lipids and other amphiphilic molecules, and additives that can be used in accordance with the invention are discussed in more detail below.
- amphiphilic molecules may be added to the aqueous solution.
- a first technique is simply to add the amphiphilic molecules to the aqueous solution outside the apparatus before introducing the aqueous solution into the chamber.
- a second technique which has particular advantage is, before introducing the aqueous solution into the chamber, to deposit the amphiphilic molecules on an internal surface of the chamber, or elsewhere in the flow path of the aqueous solution, for example in a fluidic inlet pipe connected to the inlet.
- the aqueous solution covers the internal surface during step (c) whereby the amphiphilic molecules are added to the aqueous solution.
- the aqueous solution is used to collect the amphiphilic molecules from the internal surface.
- Such deposition of the amphiphilic molecules has several advantages. It allows the formation of layer of amphiphilic molecules in the absence of large amounts of organic solvent, as would typically be present if the amphiphilic molecules were added directly to the aqueous solution.
- the deposited amphiphilic molecules can be dried.
- the aqueous solution is used to rehydrate the amphiphilic molecules. This allows the amphiphilic molecules to be stably stored in the apparatus before use. It also avoids the need for wet storage of amphiphilic molecules. Such dry storage of amphiphilic molecules increases shelf life of the apparatus.
- a first technique is simply for the aqueous solution to have a membrane protein added thereto, whereby the membrane protein is inserted spontaneously into the layer of amphiphilic molecules.
- the membrane protein may be added to the aqueous solution outside the apparatus before introducing the aqueous solution into the chamber.
- the membrane protein may be deposited on an internal surface of the chamber before introducing the aqueous solution into the chamber.
- the aqueous solution covers the internal surface during step (c), whereby the membrane protein is added to the aqueous solution.
- a second technique is for the aqueous solution to have vesicles containing the membrane protein added thereto, whereby the membrane protein is inserted on fusion of the vesicles with the layer of amphiphilic molecules.
- a third technique is to insert the membrane protein by carrying the membrane protein to the layer on a probe, for example an agar-tipped rod.
- the aqueous solution is flowed across the body to cover the recess. Formation is improved if a multi-pass technique is applied in which aqueous solution covers and uncovers the recess at least once before covering the recess for a final time. This is thought to be because at least some aqueous solution is left in the recess which assists formation of the layer in a subsequent pass.
- the pre-treatment coating is a hydrophobic fluid which assists formation of the layer by increasing the affinity of the amphiphilic molecules to the surface of the body around the recess.
- any pre-treatment that modifies the surface of the surfaces surrounding the aperture to increase its affinity to lipids may be used. Certain materials for the pre-treatment coating that can be used in accordance with the invention are discussed in more detail below.
- surfaces including either or preferably both of (a) the outermost surface of the body around the recess and (b) at least an outer part of the internal surface of the recess extending from the rim of the recess may be hydrophobic. This may be achieved by making the body with an outermost layer formed of a hydrophobic material.
- the surfaces are treated by a fluorine species, such as a fluorine radical, for example by treatment with a fluorine plasma during manufacture of the apparatus.
- a fluorine species such as a fluorine radical
- the application of the pre-treatment coating may leave excess hydrophobic fluid covering said electrode contained in the recess. This potentially insulates the electrode by reducing ionic flow, thereby reducing the sensitivity of the apparatus in measuring electrical signals.
- various different techniques may be applied to minimise this problem.
- a first technique is to apply a voltage across the electrode in the recess and a further electrode in the chamber sufficient to reduce the amount of excess hydrophobic fluid covering said electrode contained in the recess. This produces a similar effect to electro-wetting.
- the voltage is applied after flowing aqueous solution across the body to cover the recess so that aqueous solution flows into the recess. As the voltage will rupture any layer formed across the recess, subsequently the aqueous solution is flowed to uncover the recess, and then aqueous solution, having amphiphilic molecules added thereto, is flowed across the body to re-cover the recess so that a layer of the amphiphilic molecules forms across the recess.
- a second technique is to make an inner part of the internal surface of the recess hydrophilic. Typically this will be applied in combination with making the outer part of the internal surface of the recess hydrophobic. This may be achieved by making the body with an inner layer formed of a hydrophilic material and an outermost layer formed of a hydrophobic material.
- a third technique is to provide on the electrode a hydrophillic surface, for example a protective material, which repels the hydrophobic fluid applied in step (c) whilst allowing ionic conduction from the aqueous solution to the electrode.
- the protective material may be a conductive polymer, for example polypyrrole/polystyrene sulfonate.
- the protective material may be a covalently attached hydrophilic species, such as thiol-PEG.
- a method of improving the performance of an electrode in a recess in conducting electro-physiological measurements comprising depositing a conductive polymer on the electrode.
- an apparatus for conducting electro-physiological measurements comprising, a body having a recess in which an electrode is located, wherein a conductive polymer is provided on the electrode.
- the providing a conductive polymer on an electrode in a recess can improve the performance of the electrode in conducting electro-physiological measurements.
- One advantage is to improve the electrode's performance as a stable electrode for conducting electro-physiological measurements.
- a further advantage is to increase the charge reservoir available to the electrode within the recess without increasing the volume of aqueous solution contained in the recess.
- FIG. 1 is a perspective view of an apparatus
- FIG. 2 is a cross-sectional view of the apparatus of FIG. 1 , taken along line II-II in FIG. 1 , and showing the introduction of an aqueous solution;
- FIG. 3 is a cross-sectional view of the apparatus, similar to that of FIG. 2 but showing the apparatus full of aqueous solution;
- FIG. 4 is sequence of a cross-sectional, partial views of the recess in the apparatus over an electrochemical electrode modification process
- FIG. 5 is an SEM image of a recess formed by CO 2 laser drilling
- FIG. 6 is an OM image of a recess formed using photolithography
- FIGS. 7 a and 7 b are 3D and 2D LP profiles, respectively, of a recess formed using photolithography
- FIGS. 8 a and 8 b are 3D and 2D LP profiles, respectively, of a recess formed using photolithography, after electoplating;
- FIG. 9 is a cross-sectional, partial view of the recess in the apparatus with a pre-treatment coating applied
- FIGS. 10 a to 10 e are a sequence of cross-sectional, partial view of the recess in the apparatus during a method of removing excess pre-treatment coating;
- FIG. 11 is a cross-sectional, partial view of the recess in the apparatus having plural further layers in the body;
- FIG. 12 is a diagram of an electrical circuit
- FIG. 13 is a perspective view of the apparatus and electrical circuit mounted on a printed circuit board
- FIG. 14 is a diagram of an electrical circuit for acquiring plural signals in parallel
- FIG. 15 is a graph of the applied potential and current response for a dry apparatus
- FIG. 16 is a graph of the applied potential and current response for a wet apparatus
- FIG. 17 is a graph of the applied potential and current response on electro-wetting of the apparatus.
- FIG. 18 is a graph of the applied potential and current response on formation of a layer of amphiphilic molecules
- FIGS. 19 to 22 are graphs of the applied potential and current response for various different apparatuses.
- FIGS. 23 to 25 are plan views of a further layer in a modified apparatus having plural recesses
- FIGS. 26 to 28 are plan views of the substrate in the modified apparatuses having plural recesses
- FIGS. 29 and 30 are graphs of the current response for two different apparatuses having plural recesses
- FIG. 31 is a cross-sectional view of a portion of a modified apparatus
- FIG. 32 is a cross-sectional view of another modified apparatus
- FIG. 33 is a flow chart of a method of manufacture of the apparatus.
- FIGS. 34 a and 34 b are 3D and 2D surface profiles of a recess having an electrode modified by electropolymerisation of polypyrrole, measured by profilometry;
- FIG. 35 is a graph of current recorded on an array of recesses having an electrode modified by electropolymerisation of polypyrrole.
- FIG. 1 An apparatus 1 which may be used to form a layer of amphiphilic molecules is shown in FIG. 1 .
- the apparatus 1 includes a body 2 having layered construction as shown in FIGS. 2 and 3 comprising a substrate 3 of non-conductive material supporting a further layer 4 also of non-conductive material. In the general case, there may be plural further layers 4 , as described further below.
- a recess 5 is formed in the further layer 4 , in particular as an aperture which extends through the further layer 4 to the substrate 3 .
- there may be plural recesses 5 as described further below.
- the apparatus 1 further includes a cover 6 which extends over the body 2 .
- the cover 6 is hollow and defines a chamber 7 which is closed except for an inlet 8 and an outlet 9 each formed by openings through the cover 6 .
- the lowermost wall of the chamber 7 is formed by the further layer 4 in FIG. 2 , but as an alternative the further layer 4 could be shaped to provide side walls.
- aqueous solution 10 is introduced into the chamber 7 and a layer 11 of amphiphilic molecules is formed across the recess 5 separating aqueous solution 10 in the recess 5 from the remaining volume of aqueous solution in the chamber 7 .
- the apparatus includes the following electrode arrangement to allow measurement of electrical signals across the layer 11 of amphiphilic molecules.
- a chamber 7 which is closed makes it very easy to flow aqueous solution 10 into and out of the chamber 7 . This is done simply by flowing the aqueous solution 10 through the inlet 8 as shown in FIG. 2 until the chamber 7 is full as shown in FIG. 3 . During this process, gas (typically air) in the chamber 7 is displaced by the aqueous solution 10 and vented through the outlet 9 .
- gas typically air
- a simple fluidics system attached to the inlet 8 may be used. This may be as simple as a plunger, although more complicated systems may be used to improve the control.
- the chamber 7 is not necessarily closed and may be open, for example by forming the body 2 as a cup.
- the substrate 3 has a first conductive layer 20 deposited on the upper surface of the substrate 3 and extending under the further layer 4 to the recess 5 .
- the portion of the first conductive layer 20 underneath the recess 5 constitutes an electrode 21 which also forms the lowermost surface of the recess 5 .
- the first conductive layer 20 extends outside the further layer 4 so that a portion of the first conductive layer 20 is exposed and constitutes a contact 22 .
- the further layer 4 has a second conductive layer 23 deposited thereon and extending under the cover 6 into the chamber 7 , the portion of the second conductive layer 23 inside the chamber 7 constituting an electrode 24 .
- the second conductive layer 23 extends outside the cover 6 so that a portion of the second conductive layer 23 is exposed and constitutes a contact 25 .
- the electrodes 21 and 24 make electrical contact with aqueous solution in the recess 5 and chamber 7 . This allows measurement of electrical signals across the layer 11 of amphiphilic molecules by connection of an electrical circuit 26 to the contacts 22 and 25 .
- the electrical circuit 26 may have basically the same construction as a conventional circuit for performing stochastic sensing across a lipid bilayer formed in a conventional cell by the Montal & Mueller method.
- FIG. 12 An example design of the electrical circuit 26 is shown in FIG. 12 .
- the primary function of the electrical circuit 26 is to measure the electrical current signal developed between the electrodes 21 and 24 to provide a meaningful output to the user. This may be simply an output of the measured signal, but in principle could also involve further analysis of the signal.
- the electrical circuit 26 needs to be sufficiently sensitive to detect and analyse currents which are typically very low.
- an open membrane protein might typically pass current of 100 pA to 200 pA with a 1M salt solution.
- the electrode 24 in the chamber 7 is used as a reference electrode and the electrode 21 in the recess 5 is used as a working electrode.
- the electrical circuit 26 provides the electrode 24 with a bias voltage potential relative to the electrode 21 which is itself at virtual ground potential and supplies the current signal to the electrical circuit 26 .
- the electrical circuit 26 has a bias circuit 40 connected to the electrode 24 in the chamber 7 and arranged to apply a bias voltage which effectively appears across the two electrodes 21 and 24 .
- the electrical circuit 26 also has an amplifier circuit 41 connected to the electrode 21 in the recess 5 for amplifying the electrical current signal appearing across the two electrodes 21 and 24 .
- the amplifier circuit 41 consists of a two amplifier stages 42 and 43 .
- the input amplifier stage 42 connected to the electrode 21 converts the current signal into a voltage signal.
- the input amplifier stage 42 may comprise transimpedance amplifier, such as an electrometer operational amplifier configured as an inverting amplifier with a high impedance feedback resistor, of for example 500 M ⁇ , to provides the gain necessary to amplify the current signal which typically has a magnitude of the order of tens to hundreds of picoamps.
- transimpedance amplifier such as an electrometer operational amplifier configured as an inverting amplifier with a high impedance feedback resistor, of for example 500 M ⁇ , to provides the gain necessary to amplify the current signal which typically has a magnitude of the order of tens to hundreds of picoamps.
- the input amplifier stage 42 may comprise a switched integrator amplifier. This is preferred for very small signals as the feedback element is a capacitor and virtually noiseless.
- a switched integrator amplifier has wider bandwidth capability.
- the integrator does have a dead time due to the necessity to reset the integrator before output saturation occurs. This dead time may be reduced to around a microsecond so is not of much consequence if the sampling rate required is much higher.
- a transimpedance amplifier is simpler if the bandwidth required is smaller.
- the switched integrator amplifier output is sampled at the end of each sampling period followed by a reset pulse. Additional techniques can be used to sample the start of integration eliminating small errors in the system.
- the second amplifier stage 43 amplifies and filters the voltage signal output by the first amplifier stage 42 .
- the second amplifier stage 43 provides sufficient gain to raise the signal to a sufficient level for processing in a data acquisition unit 44 .
- the input voltage to the second amplifier stage 43 given a typical current signal of the order of 100 pA, will be of the order of 50 mV, and in this case the second amplifier stage 43 must provide a gain of 50 to raise the 50 mV signal range to 2.5V.
- the electrical circuit 26 includes a data acquisition unit 44 which may be a microprocessor running an appropriate program or may include dedicated hardware.
- the data acquisition unit 44 may be a card to be plugged into a computer 45 such as a desktop or laptop.
- the bias circuit 40 is simply formed by an inverting amplifier supplied with a signal from a digital-to-analog converter 46 which may be either a dedicated device or a part of the data acquisition unit 44 and which provides a voltage output dependent on the code loaded into the data acquisition unit 44 from software.
- the signals from the amplifier circuit 41 are supplied to the data acquisition card 40 through an analog-to-digital converter 47 .
- the various components of the electrical circuit 26 may be formed by separate components or any of the components may be integrated into a common semiconductor chip.
- the components of the electrical circuit 26 may be formed by components arranged on a printed circuit board. An example of this is shown in FIG. 13 wherein the apparatus 1 is bonded to a printed circuit board 50 with aluminium wires 51 connecting from the contacts 22 and 25 to tracks 52 on the printed circuit board. A chip 53 incorporating the electrical circuit 26 is also bonded to the printed circuit board 50 .
- the apparatus 1 and the electrical circuit 26 may be mounted on separate printed circuit boards.
- the electrical circuit 26 is modified essentially by replicating the amplifier circuit 41 and A/D converter 47 for each electrode 21 to allow acquisition of signals from each recess 5 in parallel.
- the input amplifier stage 42 comprises switched integrators then those would require a digital control system to handle the sample-and-hold signal and reset integrator signals.
- the digital control system is most conveniently configured on a field-programmable-gate-array device (FPGA).
- FPGA field-programmable-gate-array device
- the FPGA can incorporate processor-like functions and logic required to interface with standard communication protocols i.e. USB and Ethernet.
- FIG. 14 shows a possible architecture of the electrical circuit 26 and is arranged as follows.
- the respective electrodes 21 of the apparatus 1 are connected to the electrical circuit 26 by an interconnection 55 , for example the aluminium wires 51 and the printed circuit board in the arrangement of FIG. 13 .
- the amplifier circuits 41 may be formed in one or more amplifier chips 56 having plural channels.
- the signals from different electrodes 21 may be on separate channels or multiplexed together on the same channel.
- the outputs of the one or more amplifier chips 56 are supplied via the A/D converter 47 to a programmable logic device 57 for receiving the signal on each channel.
- the programmable logic device 57 might operate at a speed of the order of 10 Mbits/s.
- the programmable logic device 57 is connected via an interface 58 , for example a USB interface, to a computer 59 to supply the signals to the computer 59 for storage, display and further analysis.
- the apparatus 1 may be enclosed in a Faraday cage to reduce interference.
- the materials for each component of apparatus 1 are determined by the properties required to enable the component to function correctly during operation, but the cost and manufacturing throughput are also considered. All materials should be chosen to provide sufficient mechanical strength to allow robust handling, and surfaces compatible with bonding to the subsequent layers.
- the material of the substrate 3 is chosen to provide a rigid support for the remainder of the apparatus 1 .
- the material is also chosen to provide a high resistance and low capacitance electrical insulation between adjacent electrodes 21 when there are plural recesses 5 .
- Possible materials include without limitation: polyester (eg Mylar), or another polymer; or silicon, silicon nitride, or silicon oxide.
- the substrate may comprise a silicon wafer with a thermally grown oxide surface layer.
- the material of the further layer 4 (or in the general case layers) are chosen to provide a high resistance and low capacitance electrical insulation between the electrodes 21 and 24 and also, when there are plural recesses 5 , between the electrodes 21 and 24 of adjacent recesses 5 .
- the surface of the further layer 4 should be chemically stable both to the pre-treatment coating applied before operation (as discussed below) and to the aqueous solution 10 .
- the further layer 4 should be mechanically robust in order to maintain its structural integrity and coverage of the first conductive layer 20 , and should be suitable for subsequent attachment of the cover 6 .
- photoresist eg SU8 photoresist or Cyclotene
- polycarbonate 6 ⁇ m thick film
- PVC 7 ⁇ m thick film
- polyester 50 ⁇ m thick film
- adhesive backed polyester 25 ⁇ m and 50 ⁇ m thick film
- thermal laminating films eg Magicard 15 ⁇ m thick and Murodigital 35 ⁇ m
- screen-printed dielectric ink eg Magicard 15 ⁇ m thick and Murodigital 35 ⁇ m
- surfaces including (a) the outermost surface of the body 2 around the recess and (b) the outer part of the internal surface of the recess 5 extending from the rim of the recess 5 are hydrophobic. This assists in the spreading of the pre-treatment coating and therefore also formation of a lipid bilayer.
- a fluorine species is any substance capable of modifying the surfaces to provide a fluorine-containing layer.
- the fluorine species is preferably one containing fluorine radicals.
- the modification may be achieved by treating the body 2 with a fluorine plasma, for example a CF 4 during manufacture.
- the material of the electrodes 21 and 24 should provide an electrochemical electrode in contact with the aqueous solution 10 , enabling measurement of low currents, and should be stable to the pre-treatment coating and aqueous solution 10 .
- the material of the remainder of the conductive layers 20 and 23 (usually but not necessarily the same as the electrodes 21 and 24 ) also provides electrical conductance from the electrodes to the contacts 22 and 25 .
- the first conductive layers 20 will also accept bonding of the further layers 4 .
- the conductive layers 20 and 23 can be constructed with plural overlapping layers and/or an appropriate surface treatment.
- One possible material is platinum, coated with silver at the area exposed to the test solution and then silver chloride formed on top of the silver.
- Possible materials for the first conductive layer 20 include without limitation: Silver/silver chloride electrode ink; silver with or without a surface layer, for example of silver chloride formed by chloridisation or of silver fluoride formed by fluoridisation; gold with or without redox couple in solution; platinum with or without redox couple in solution; ITO with and without redox couple in solution; gold electrochemically coated with conductive polymer electrolyte; or platinum electrochemically coated with conductive polymer electrolyte.
- Possible materials for the second conductive layer 23 include without limitation: silver/silver chloride electrode ink; silver wire; or chloridised silver wire.
- Some specific examples of include: the substrate 3 being silicon and the conductive layer 20 being a metal conductor (diffusion or polysilicon wires are poor methods) buried in a silicon oxide insulating layer (e.g. using typical semiconductor fabrication technology); the substrate 3 being glass and the conductive layer 20 being metal conductors (e.g using typical LCD display technology); or the substrate 3 being a polymeric substrates and the conductive layer 20 being an ablated metal or printed conductor (e.g. using typical glucose biosensor technology).
- the requirements for the material of the cover 6 are to be easily attached to create a seal for the chamber 7 , to be compatible with both the pre-treatment coating and the aqueous solution 10 .
- the following are possible materials, together with thicknesses which have been successfully employed experimentally, although these thicknesses are not limitative: silicone rubber, 0.5, 1.0, 2.0 mm thick; polyester, 0.5 mm thick; or PMMA (acrylic) 0.5 mm to 2 mm thick.
- the layered construction of the apparatus 1 is simple and easy to form by a variety of methods.
- Three different fabrication technologies which have actually been applied are: lamination of polymer films; printed circuit board manufacture with high resolution solder mask formation and photolithography using silicon wafers or glass.
- the substrate 3 is a 250 ⁇ m thick polyester sheet (Mylar), and the first conductive layer 20 is deposited by either: screen printing silver/silver chloride electrode ink; adhesion of metal foil; or vapour deposition (sputtering or evaporation).
- the further layer 4 is then laminated onto the substrate 3 by either: a pressure-sensitive adhesive; a thermally activated adhesive; or using the wet silver/silver chloride ink as the adhesive painted directly onto the dielectric before lamination (referred to as “painted electrodes”).
- the aperture in the further layer 4 that forms the recess 5 is created with 5-100 ⁇ m diameter either before or after lamination to the substrate 3 by either: electrical discharge (sparking); or laser drilling, for example by an excimer, solid state or CO 2 laser.
- An apparatus created by lamination of polymer films sometimes requires an additional sparking step to activate the electrodes prior to use.
- the second conductive layer 23 is formed on top of the further layer 4 by screen printing.
- the cover 6 is laminated on top using pressure sensitive adhesive.
- the substrate 3 is a silicon wafer with an oxide surface layer.
- the first conductive layer 20 is formed by gold, silver, chloridised silver, platinum or ITO deposited onto the substrate 3 .
- Photoresist eg SU8
- the recess 5 is formed with 5-100 ⁇ m diameter by removal of the photoresist following UV exposure using a mask to define the shape of the recess 5 .
- the second conductive layer 23 is formed on top of the further layer 4 , for example by screen printing.
- the cover 6 is laminated on top using pressure sensitive adhesive.
- the electrodes 21 and 24 will now be discussed further.
- the electrodes 21 and 24 should operate at the required low current levels with a low over-potential and maintain their electrode potential value over the course of the measurement. Further, the electrodes 21 and 24 should introduce a minimum amount of noise into the current signal.
- Possible materials for the electrodes 21 and 24 include without limitation: Silver/silver chloride electrode ink; silver with or without a surface layer, for example of silver chloride formed by chloridisation or of silver fluoride formed by fluoridisation; gold with or without redox couple in solution; platinum with or without redox couple in solution; ITO with and without redox couple in solution; palladium hydride, gold electrochemically coated with conductive polymer electrolyte; or platinum electrochemically coated with conductive polymer electrolyte.
- Silver is a good choice for the material of electrodes 21 and 24 but is difficult to incorporate in a silicon wafer manufacturing process due to its tendency to undergo oxidation on exposure to light, air and high temperatures.
- an inert conductive material eg Pt or Au
- Electroplating of silver may be achieved, for example, using a modified version of the method of Polk et al., “Ag/AgCl microelectrodes with improved stability for microfluidics”, Sensors and Actuators B 114 (2006) 239-247.
- a plating solution is prepared by addition of 0.41 g of silver nitrate to 20 ml of 1M ammonium hydroxide solution. This is rapidly shaken to avoid precipitation of the insoluble silver oxide, and to facilitate the formation of the diammine silver complex. The solution is always fresh to avoid fall in plating efficiency.
- the plating is performed using conventional equipment, connecting the electrode 21 as the cathode and using a platinum electrode is used as the anode.
- a potential of ⁇ 0.58V is applied to the cathode, with the anode being held at ground potential, whereas in the case of plating on Au electrodes, the potential is held at ⁇ 0.48V with respect to ground.
- a target charge of 5.1 ⁇ 10 3 C/m 2 has been found empirically to result in a silver deposition of between 1 ⁇ m and 2 ⁇ m for a 100 ⁇ m diameter electrode, typically taking of the order of 60 s.
- the layer 4 is formed from a naturally hydrophobic material (eg SU8 photoresist) and in order to ensure uniform wetting of the recess, desirably the degree of hydrophilicity can be increased.
- a first method is application of a lipid to the surface of the layer 4 , so that the lipid acts as a surfactant, facilitating the entry of the plating solution.
- a second method is exposure of the layer 4 to oxygen plasma which activates the material of the layer and produces hydrophilic functional groups. This produces a well defined hydrophilic and clean surface.
- a third method is to add ethanol to the plating solution.
- the outer surface of the electrode is desirably converted to a halide, in order for the electrode 21 to function efficiently as a provider of a stable reference potential.
- the halide used is chloride, since the conversion of silver to silver chloride is relatively straightforward to achieve, for example by electrolysis in a solution of hydrochloric acid.
- Alternative chemical methods avoiding the use of a potentially corrosive acid which may affect the surface condition of the layer 4 include a) sweeping voltammetry in 3M sodium chloride solution, and b) a chemical etching by immersion of the electrode 21 in 50 mM ferric chloride solution.
- An alternative halogen for the halidisation is fluorine.
- the choice of fluorine has the significant advantage that the silver fluoride layer can be formed in the same step as modification of surfaces (a) and (b) of the body 2 to make them hydrophobic, as discussed above. For example this may be achieved during manufacture of the apparatus 1 by treatment of the body 2 by a fluorine plasma for example a CF 4 plasma. This is effective to modify the surfaces of the body 2 , particularly in the case that the layer 4 is a photoresist such as SU8 to achieve a sufficient degree of hydrophobicity to support the formation of a stable lipid bilayer. At the same time exposure to the fluorine plasma converts the metal of the electrode 21 into an outer layer of metal fluoride.
- the electrode 21 may be electrochemically modified to change the surface-type. This allows use of additional materials with good bulk properties but poor surface properties, such as gold. Possible electrochemical surface modifications include without limitation: silver electroplating; electrochemical chloridisation of silver; electropolymerisation of a polymer/polyelectrolyte.
- FIG. 4 one possible sequence of modification is shown in FIG. 4 in which a coating 37 of silver is formed on the electrode 21 formed of gold or platinum by electrochemical deposition. Electroplating may typically be performed in 0.2M AgNO 2 , 2M KI, 0.5 mM Na 2 S 2 O 3 at ⁇ 0.48V using a standard single liquid junction Ag/AgCl reference electrode and a platinum counter electrode. A typical thickness of the coating 37 is estimated to be 750 nm with a deposition time of about 50 s and about 50 ⁇ C charge passed. Subsequently a chloridised layer 38 is formed by chloridisation, typically at +150 mV in 0.1M HCl for 30 s.
- the conductive polymer may be any polymer which is conductive.
- a suitable conductive polymer will have mobile charge carriers.
- a conductive polymer will have a backbone having delocalised electrons which are capable of acting as charge carriers, allowing the polymer to conduct.
- the conductive polymer may be doped to increase its conductivity, for example by a redox process or by electrochemical doping.
- Suitable conductive polymers include, without limitation: polypyrroles, polyacetylenes, polythiophenes, polyphenylenes, polyanilines, polyfluorenes, poly(3-alkylthiophene)s, polytetrathiafulvalenes, polynaphthalenes, poly(p-phenylene sulfide)s, polyindoles, polythionines, polyethylenedioxythiophenes, and poly(para-phenylene vinylene)s.
- One possible conductive polymer is a polypyrrole, which may be doped, for example with polystyrene sulfonate. This may be deposited, for example, on an electrode 21 of gold by electrooxidizing an aqueous solution of 0.1M pyrrole+90 mM polystyrene sulfonate in 0.1M KCl at +0.80V vs. Ag/AgCl reference electrode.
- the estimated thickness of polymer deposited is 1 ⁇ m at 30 ⁇ C, based on a assumption that 40 mC/cm 2 of charge produces a film of thickness around 0.1 ⁇ m.
- the polymerization process can be represented as follows, where PE stands for polystyrene sulfonate:
- One advantage of using a conductive polymer deposited on an inert electrode, such as polypyrrole doped with polystyrene, electropolymerised onto gold or platinum, is to improve the electrode's performance as a stable electrode for conducting electrophysiological measurements.
- a further advantage is to increase the charge reservoir available to the electrode within the recess without increasing the volume of aqueous solution contained in the recess.
- a conductive polymer on the electrode 21 in the recess 5 of the apparatus 1 include but are not limited to control of the hydrophilic nature of the electrode surface to aid wetting of the electrode surface by the aqueous buffer solution and similarly prevention of blocking of the electrode by the chemical pre-treatment prior to bilayer formation.
- FIGS. 34 a and 34 b are 3D and 2D surface profiles of an example electrode modified by electropolymerisation of polypyrrole, measured by profilometry.
- the thickness of electrochemically deposited polymer film in this example is about 2 ⁇ m.
- FIG. 35 shows the current recorded on an array of recesses modified by electropolymerisation of polypyrrole, showing stable lipid bilayers and single molecule detection of cyclodextrin from inserted protein pores.
- an alternative to the second conductive layer 23 is to form an electrode in the chamber 7 simply by insertion through the cover 6 of a conductive member, such as a chloridised silver wire.
- OM optical microscopy
- SEM scanning electron microscopy
- LP laser profilometry
- FIG. 5 shows an SEM image of a recess 5 formed by drilling with a CO 2 laser in an apparatus 1 formed by lamination of polymer layers, with subsequent application of electrical discharge to activate the electrode 21 .
- the image illustrates that the geometry of the recess 5 is poorly defined using this method of formation, with considerable surface damage therearound and variability in diameter, although it is hoped this may be improved through optimisation of the laser characteristics.
- FIG. 6 shows an OM image of a recess 5 formed using photolithography of a further layer 4 of SU8 photoresist over an electrode 21 of vapour deposited gold on a substrate 3 of silicon.
- FIGS. 7 a and 7 b are 3D and 2D LP profiles of a similarly manufactured recess 5 .
- FIGS. 8 a and 8 b are 3D and 2D LP profiles of the same recess 5 after electroplating to form a coating 38 of silver.
- Excimer laser methods also produce a controlled geometry similar to photolithography.
- step S 1 the wafer is cleaned.
- step S 2 the wafer is subjected to a HF dif to improve adhesion of metals and resist. Typical conditions are a 3 minute dip in 10:1 buffered oxide etch.
- step S 3 the wafer is subjected to a bake as a dehydration step. Typical conditions are baking for 1 hour at 200° C. in an oven.
- step S 4 photoresist is spun onto the wafer which is then subjected to UV light to form the desired pattern.
- the conductive layers 20 are deposited, for example consisting of successive layers of Cr and Au. Typically of respective thicknesses 50 nm and 300 nm.
- step S 6 the resist is removed for example by soaking in acetone.
- step S 7 photoresist adhesion is improved by the application of an O 2 plasma and dehydration bake for example in an oven.
- step S 8 the wafer has applied thereto photoresist which is then subjected to UV exposure to form the layers 4 and recesses, for example SU8-10 with a thickness of 20 m.
- step S 9 an inspection and measurement of the recesses is performed.
- step S 10 the surface is prepared for plating by performing an O2 plasma descum.
- step S 11 silver plating of the electrode is performed, as described above, for example to form a plating thickness of 1.5 ⁇ m.
- step S 12 the wafer is diced to form the bodies 2 of separate apparatuses 1 .
- the bodies 2 are treated by a CF 4 plasma which modifies the surfaces of the body 2 and the electrode 21 as discussed above.
- a typical exposure is for 12 minutes at 70 W and 160 mTorr.
- the amphiphilic molecules are typically a lipid.
- the layer is a bilayer formed from two opposing monolayers of lipid.
- the two monolayers of lipids are arranged such that their hydrophobic tail groups face towards each other to form a hydrophobic interior.
- the hydrophilic head groups of the lipids face outwards towards the aqueous environment on each side of the bilayer.
- the bilayer may be present in a number of lipid phases including, but not limited to, the liquid disordered phase (fluid lamellar), liquid ordered phase, solid ordered phase (lamellar gel phase, interdigitated gel phase) and planar bilayer crystals (lamellar sub-gel phase, lamellar crystalline phase).
- lipids that form a lipid bilayer may be used.
- the lipids are chosen such that a lipid bilayer having the required properties, such as surface charge, ability to support membrane proteins, packing density or mechanical properties, is formed.
- the lipids can comprise one or more different lipids.
- the lipids can contain up to 100 lipids.
- the lipids preferably contain 1 to 10 lipids.
- the lipids may comprise naturally-occurring lipids and/or artificial lipids.
- the lipids typically comprise a head group, an interfacial moiety and two hydrophobic tail groups which may be the same or different.
- Suitable head groups include, but are not limited to, neutral head groups, such as diacylglycerides (DG) and ceramides (CM); zwitterionic head groups, such as phosphatidylcholine (PC), phosphatidylethanolamine (PE) and sphingomyelin (SM); negatively charged head groups, such as phosphatidylglycerol (PG); phosphatidylserine (PS), phosphatidylinositol (PI), phosphatic acid (PA) and cardiolipin (CA); and positively charged headgroups, such as trimethylammonium-Propane (TAP).
- neutral head groups such as diacylglycerides (DG) and ceramides (CM)
- zwitterionic head groups such as phosphatidylcholine (PC), phosphatidylethanolamine (PE
- Suitable interfacial moieties include, but are not limited to, naturally-occurring interfacial moieties, such as glycerol-based or ceramide-based moieties.
- Suitable hydrophobic tail groups include, but are not limited to, saturated hydrocarbon chains, such as lauric acid (n-Dodecanolic acid), myristic acid (n-Tetradecononic acid), palmitic acid (n-Hexadecanoic acid), stearic acid (n-Octadecanoic) and arachidic (n-Eicosanoic); unsaturated hydrocarbon chains, such as oleic acid (cis-9-Octadecanoic); and branched hydrocarbon chains, such as phytanoyl.
- the length of the chain and the position and number of the double bonds in the unsaturated hydrocarbon chains can vary.
- the length of the chains and the position and number of the branches, such as methyl groups, in the branched hydrocarbon chains can vary.
- the hydrophobic tail groups can be linked to the interfacial moiety as an ether or an ester.
- the lipids can also be chemically-modified.
- the head group or the tail group of the lipids may be chemically-modified.
- Suitable lipids whose head groups have been chemically-modified include, but are not limited to, PEG-modified lipids, such as 1,2-Diacyl-sn-Glycero-3-Phosphoethanolamine-N-[Methoxy(Polyethylene glycol)-2000]; functionionalised PEG Lipids, such as 1,2-Distearoyl-sn-Glycero-3 Phosphoethanolamine-N-[Biotinyl(Polyethylene Glycol)2000]; and lipids modified for conjugation, such as 1,2-Dioleoyl-sn-Glycero-3-Phosphoethanolamine-N-(succinyl) and 1,2-Dipalmitoyl-sn-Glycero-3-Phosphoethanolamine-N-(Biotinyl).
- Suitable lipids whose tail groups have been chemically-modified include, but are not limited to, polymerisable lipids, such as 1,2-bis(10,12-tricosadiynoyl)-sn-Glycero-3-Phosphocholine; fluorinated lipids, such as 1-Palmitoyl-2-(16-Fluoropalmitoyl)-sn-Glycero-3-Phosphocholine; deuterated lipids, such as 1,2-Dipalmitoyl-D62-sn-Glycero-3-Phosphocholine; and ether linked lipids, such as 1,2-Di-O-phytanyl-sn-Glycero-3-Phosphocholine.
- polymerisable lipids such as 1,2-bis(10,12-tricosadiynoyl)-sn-Glycero-3-Phosphocholine
- fluorinated lipids such as 1-Palmit
- the lipids typically comprise one or more additives that will affect the properties of the lipid bilayer.
- Suitable additives include, but are not limited to, fatty acids, such as palmitic acid, myristic acid and oleic acid; fatty alcohols, such as palmitic alcohol, myristic alcohol and oleic alcohol; sterols, such as cholesterol, ergosterol, lanosterol, sitosterol and stigmasterol; lysophospholipids, such as 1-Acyl-2-Hydroxy-sn-Glycero-3-Phosphocholine; and ceramides.
- the lipid preferably comprises cholesterol and/or ergosterol when membrane proteins are to be inserted into the lipid bilayer.
- lipids are commonly used to form bilayers, it is expected that in general the method is applicable to any amphiphilic molecules which may form a layer.
- aqueous solution 10 in general a wide range of aqueous solutions 10 that are compatible with the formation of a layer 11 of amphiphilic molecules may be used.
- the aqueous solution 10 is typically a physiologically acceptable solution.
- the physiologically acceptable solution is typically buffered to a pH of 3 to 11.
- the pH of the aqueous solution 10 will be dependent on the amphiphilic molecules used and the final application of the layer 11 .
- Suitable buffers include without limitation: phosphate buffered saline (PBS); N-2-Hydroxyethylpiperazine-N′-2-Ethanesulfonic Acid (HEPES) buffered saline; Piperazine-1,4-Bis-2-Ethanesulfonic Acid (PIPES) buffered saline; 3-(n-Morpholino)Propanesulfonic Acid (MOPS) buffered saline; and Tris(Hydroxymethyl)aminomethane (TRIS) buffered saline.
- PBS phosphate buffered saline
- HPES N-2-Hydroxyethylpiperazine-N′-2-Ethanesulfonic Acid
- PPES Piperazine-1,4-Bis-2-Ethanesulfonic Acid
- MOPS 3-(n-Morpholino)Propanesulfonic Acid
- TMS Tris
- the method of using the apparatus 1 is as follows.
- a pre-treatment coating 30 is applied to the body 2 across the recess 5 , as shown in FIG. 9 .
- the pre-treatment coating 30 is a hydrophobic fluid which modifies the surface of the body 2 surrounding the recess 5 to increase its affinity to the amphiphilic molecules.
- the pre-treatment coating 30 is typically an organic substance, usually having long chain molecules, in an organic solvent.
- Suitable organic substances include without limitation: n-decane, hexadecane, isoecoisane, squalene, fluoroinated oils (suitable for use with fluorinated lipids), alkyl-silane (suitable for use with a glass membrane) and alkyl-thiols (suitable for use with a metallic membrane).
- Suitable solvents include but are not limited to: pentane, hexane, heptane, octane, decane, and toluene.
- the material might typically be 0.1 ⁇ l to 10 ⁇ l of 0.1% to 50% (v/v) hexadecane in pentane or another solvent, for example 2 ⁇ l of 1% (v/v) hexadecane in pentane or another solvent, in which case lipid, such as diphantytanoyl-sn-glycero-3-phosphocholine (DPhPC), might be included at a concentration of 0.6 mg/ml.
- lipid such as diphantytanoyl-sn-glycero-3-phosphocholine (DPhPC)
- the pre-treatment coating 30 may be applied in any suitable manner, for example simply by capillary pipette.
- the pre-treatment coating 30 may be applied before or after the cover 6 is attached to the apparatus 1 .
- the precise volume of material of the pre-treatment coating 30 required depends on the size of the recess 5 , the formulation of the material, and the amount and distribution of the when it dries around the aperture. In general increasing the amount (by volume and/or by concentration) improves the effectiveness, although excessive material can cover the electrode 21 as discussed below. As the diameter of the recess 5 is decreased, the amount of material of the pre-treatment coating 30 required also varies. The distribution of the pre-treatment coating 30 can also affect effectiveness, this being dependent on the method of deposition, and the compatibility of the membrane surface chemistry. Although the relationship between the pre-treatment coating 30 and the ease and stability of layer formation is complex, it is straightforward to optimise the amount by routine trial and error. In another method the chamber 7 can be completely filled by pre-treatment in solvent followed by removal of the excess solvent and drying with a gas flow.
- the pre-treatment coating 30 is applied across the recess 5 .
- the pre-treatment coating 30 covers the surface of the body 2 around the recess 5 .
- the pre-treatment coating 30 also extends over the rim of the recess 5 and desirably covers at least the outermost portion of the side walls of the recess 5 . This assists with formation of the layer 11 of amphiphilic molecules across the recess 5 .
- the pre-treatment coating 30 also has a natural tendency during application to cover the electrode 21 . This is undesirable as the pre-treatment coating 30 reduces the flow of current to the electrode 21 and therefore reduces the sensitivity of measurement of electrical signals, in the worst case preventing any measurement at all. A number of different techniques may be employed to reduce or avoid this problem, and will be discussed after the description of forming the layer 11 of amphiphilic molecules.
- the aqueous solution 10 is flowed across the body 2 to cover the recess 5 as shown in FIG. 3 .
- This step is performed with the amphiphilic molecules added to the aqueous solution 10 . It has been demonstrated that, with an appropriate pre-treatment coating 30 this allows the formation of the layer 11 of amphiphilic molecules across the recess 5 . Formation is improved if a multi-pass technique is applied in which aqueous solution 10 covers and uncovers the recess 5 at least once before covering the recess 5 for a final time. This is thought to be because at least some aqueous solution is left in the recess 5 which assists formation of the layer 11 in a subsequent pass.
- the formation of the layer 11 is reliable and repeatable. This is despite the fact that the practical technique of flowing aqueous solution 10 across the body 2 through the chamber 7 is very easy to perform. Formation of the layer 11 may be observed by monitoring of the resultant electrical signals across the electrodes 21 and 24 , as described below. Even if a layer 11 fails to form it is a simple matter to perform another pass of the aqueous solution 10 . Such reliable formation of a layer 11 of amphiphilic molecules using a simple method and a relatively simple apparatus 1 is a particular advantage of the present invention.
- the layers 11 of amphiphilic molecules are of high quality, in particular being suitable for high sensitivity biosensor applications such as stochastic sensing and single channel recording.
- the layers 11 have high resistance providing highly resistive electrical seals, having an electrical resistance of 1 G ⁇ or more, typically at least 100 G ⁇ . which, for example, enable high-fidelity stochastic recordings from single protein pores.
- the volume of aqueous solution 10 is sufficient to allow stable continuous dc current measurement through membrane proteins inserted in the layer.
- a first technique is simply to add the amphiphilic molecules to the aqueous solution 10 outside the apparatus 1 before introducing the aqueous solution 10 into the chamber 7 .
- a second technique which has particular advantage is, before introducing the aqueous solution 10 into the chamber 7 , to deposit the amphiphilic molecules on an internal surface of the chamber 7 , or on an internal surface elsewhere in the flow path of the aqueous solution 10 into the chamber 7 , for example in a fluidic inlet pipe connected to the inlet.
- the amphiphilic molecules can be deposited on any one or more of the internal surfaces of the chamber 7 , including a surface of the further layer 4 or of the cover 6 .
- the aqueous solution 10 covers the internal surface during its introduction, whereby the amphiphilic molecules are added to the aqueous solution 10 . In this manner, the aqueous solution 10 is used to collect the amphiphilic molecules from the internal surface.
- the aqueous solution 10 may cover the amphiphilic molecules and the recess 5 in any order but preferably covers the amphiphilic molecules first. If the amphiphilic molecules are to be covered first, the amphiphilic molecules are deposited along the flow path between the inlet 8 and the recess 5 .
- Any method may be used to deposit the lipids on an internal surface of the chamber 7 . Suitable methods include, but are not limited to, evaporation or sublimation of a carrier solvent, spontaneous deposition of liposomes or vesicles from a solution and direct transfer of the dry lipid from another surface.
- An apparatus 1 having lipids deposited on an internal surface may be fabricated using methods including, but not limited to, drop coating, various printing techniques, spin-coating, painting, dip coating and aerosol application.
- the deposited amphiphilic molecules are preferably dried.
- the aqueous solution 10 is used to rehydrate the amphiphilic molecules. This allows the amphiphilic molecules to be stably stored in the apparatus 1 before use. It also avoids the need for wet storage of amphiphilic molecules. Such dry storage of amphiphilic molecules increases shelf life of the apparatus. Even when dried to a solid state, the amphiphilic molecules will typically contain trace amounts of residual solvent.
- Dried lipids are preferably lipids that comprise less than 50 wt % solvent, such as less than 40 wt %, less than 30 wt %, less than 20 wt %, less than 15 wt %, less than 10 wt % or less than 5 wt % solvent.
- a membrane protein is inserted into the layer 11 of amphiphilic molecules. There are several techniques for achieving this.
- a first technique is simply for the aqueous solution 10 to have a membrane protein added thereto, whereby the membrane protein is inserted spontaneously into the layer 11 of amphiphilic molecules after a period of time.
- the membrane protein may be added to the aqueous solution 10 outside the apparatus 1 before introducing the aqueous solution 10 into the chamber 7 .
- the membrane protein may be added after formation of the layer 11 .
- Another way of adding the membrane protein to the aqueous solution 10 is to deposit it on an internal surface of the chamber 7 before introducing the aqueous solution 10 into the chamber 7 .
- the aqueous solution 10 covers the internal surface during its introduction, whereby the membrane protein is added to the aqueous solution 10 and subsequently will spontaneously insert into layer 11 .
- the membrane proteins may be deposited on any one or more of the internal surfaces of the chamber 7 , including a surface of the further layer 4 or of the cover 6 .
- the membrane proteins can be deposited on the same or different internal surface as the amphiphilic molecules (if also deposited).
- the amphiphilic molecules and the membrane proteins may be mixed together.
- Any method may be used to deposit the membrane proteins on an internal surface of the chamber 7 . Suitable methods include, but are not limited to, drop coating, various printing techniques, spin-coating, painting, dip coating and aerosol application.
- the membrane proteins are preferably dried.
- the aqueous solution 10 is used to rehydrate the membrane proteins. Even when dried to a solid state, the membrane proteins will typically contain trace amounts of residual solvent.
- Dried membrane proteins are preferably membrane proteins that comprise less than 20 wt % solvent, such as less than 15 wt % , less than 10 wt % or less than 5 wt % solvent.
- a second technique is for the aqueous solution 10 to have vesicles containing the membrane protein added thereto, whereby the membrane protein is inserted on fusion of the vesicles with the layer 11 of amphiphilic molecules.
- a third technique is to insert the membrane protein by carrying the membrane protein to the layer 11 on a probe, for example an agar-tipped rod, using the techniques disclosed in WO-2006/100484.
- a probe may assist in selectively inserting different membrane proteins in different layers 11 , in the case that the apparatus has an array of recesses. However, this requires modification to the apparatus 1 to accommodate the probe.
- membrane proteins that insert into a lipid bilayer may be deposited.
- the membrane proteins may be naturally-occurring proteins and/or artificial proteins.
- Suitable membrane proteins include, but are not limited to, ⁇ -barrel membrane proteins, such as toxins, porins and relatives and autotransporters; membrane channels, such as ion channels and aquaporins; bacterial rhodopsins; G-protein coupled receptors; and antibodies.
- non-constitutive toxins include hemolysin and leukocidin, such as Staphylococcal leukocidin.
- porins include anthrax protective antigen, maltoporin, OmpG, OmpA and OmpF.
- autotransporters include the NalP and Hia transporters.
- ion channels include the NMDA receptor, the potassium channel from Streptomyces lividans (KcsA), the bacterial mechanosensitive membrane channel of large conductance (MscL), the bacterial mechanosensitive membrane channel of small conductance (MscS) and gramicidin.
- G-protein coupled receptors include the metabotropic glutamate receptor.
- the membrane protein can also be the anthrax protective antigen.
- the membrane proteins preferably comprise ⁇ -hemolysin or a variant thereof.
- the ⁇ -hemolysin pore is formed of seven identical subunits (heptameric).
- the polynucleotide sequence that encodes one subunit of a-hemolysin is shown in SEQ ID NO: 1.
- the full-length amino acid sequence of one subunit of a-hemolysin is shown in SEQ ID NO: 2.
- the first 26 amino acids of SEQ ID NO: 2 correspond to the signal peptide.
- the amino acid sequence of one mature subunit of ⁇ -hemolysin without the signal peptide is shown in SEQ ID NO: 3.
- SEQ ID NO: 3 has a methionine residue at position 1 instead of the 26 amino acid signal peptide that is present in SEQ ID NO: 2.
- a variant is a heptameric pore in which one or more of the seven subunits has an amino acid sequence which varies from that of SEQ ID NO: 2 or 3 and which retains pore activity.
- 1, 2, 3, 4, 5, 6 or 7 of the subunits in a variant ⁇ -hemolysin may have an amino acid sequence that varies from that of SEQ ID NO: 2 or 3.
- the seven subunits within a variant pore are typically identical but may be different.
- the variant may be a naturally-occurring variant which is expressed by an organism, for instance by a Staphylococcus bacterium.
- Variants also include non-naturally occurring variants produced by recombinant technology. Over the entire length of the amino acid sequence of SEQ ID NO: 2 or 3, a variant will preferably be at least 50% homologous to that sequence based on amino acid identity. More preferably, the subunit polypeptide is at least 80%, at least 90%, at least 95%, at least 98%, at least 99% homologous based on amino acid identity to the amino acid sequence of SEQ ID NO: 2 or 3 over the entire sequence.
- Amino acid substitutions may be made to the amino acid sequence of SEQ ID NO: 2 or 3, for example a single amino acid substitution may be made or two or more substitutions may be made. Conservative substitutions may be made, for example, according to the following table. Amino acids in the same block in the second column and preferably in the same line in the third column may be substituted for each other:
- Non-conservative substitutions may also be made at one or more positions within SEQ ID NO: 2 or 3, wherein the substituted residue is replaced with an amino acid of markedly different chemical characteristics and/or physical size.
- One example of a non-conservative substitution that may be made is the replacement of the lysine at position 34 in SEQ ID NO: 2 and position 9 in SEQ ID NO: 3 with cysteine (i.e. K34C or K9C).
- Another example of a non-conservative substitution that may be made is the replacement of the asparagine residue at position 43 of SEQ ID NO: 2 or position 18 of SEQ ID NO: 3 with cysteine (i.e. N43C or N17C).
- cysteine residues in SEQ ID NO: 2 or 3 provides thiol attachment points at the relevant positions. Similar changes could be made at all other positions, and at multiple positions on the same subunit.
- One or more amino acid residues of the amino acid sequence of SEQ ID NO: 2 or 3 may alternatively or additionally be deleted. Up to 50% of the residues residues may be deleted, either as a contiguous region or multiple smaller regions distributed throughout the length of the amino acid chain.
- Variants can include subunits made of fragments of SEQ ID NO: 2 or 3. Such fragments retain their ability to insert into the lipid bilayer. Fragments can be at least 100, such as 150, 200 or 250, amino acids in length. Such fragments may be used to produce chimeric pores. A fragment preferably comprises the ⁇ -barrel domain of SEQ ID NO: 2 or 3.
- Variants include chimeric proteins comprising fragments or portions of SEQ ID NO: 2 or 3.
- Chimeric proteins are formed from subunits each comprising fragments or portions of SEQ ID NO: 2 or 3.
- the ⁇ -barrel part of chimeric proteins are typically formed by the fragments or portions of SEQ ID NO: 2 or 3.
- One or more amino acid residues may alternatively or additionally be inserted into, or at one or other or both ends of, the amino acid sequence SEQ ID NO: 2 or 3. Insertion of one, two or more additional amino acids to the C terminal end of the peptide sequence is less likely to perturb the structure and/or function of the protein, and these additions could be substantial, but preferably peptide sequences of up to 10, 20, 50, 100 or 500 amino acids or more can be used. Additions at the N terminal end of the monomer could also be substantial, with one, two or more additional residues added, but more preferably 10, 20, 50, 500 or more residues being added. Additional sequences can also be added to the protein in the trans-membrane region, between amino acid residues 119 and 139 of SEQ ID NO: 3.
- a carrier protein may be fused to an amino acid sequence according to the invention.
- Standard methods in the art may be used to determine homology.
- the UWGCG Package provides the BESTFIT program which can be used to calculate homology, for example used on its default settings (Devereux et al (1984) Nucleic Acids Research 12, p 387-395).
- the PILEUP and BLAST algorithms can be used to calculate homology or line up sequences (such as identifying equivalent residues or corresponding sequences (typically on their default settings)), for example as described in Altschul S. F. (1993) J Mol Evol 36:290-300; Altschul, S. F et al (1990) J Mol Biol 215:403-10.
- Software for performing BLAST analyses is publicly available through the National Center for Biotechnology Information (https://www.ncbi.nlm.nih.gov/).
- the membrane proteins can be labelled with a revealing label.
- the revealing label can be any suitable label which allows the proteins to be detected. Suitable labels include, but are not limited to, fluorescent molecules, radioisotopes, e.g. 125I, 35S, enzymes, antibodies, polynucleotides and linkers such as biotin.
- the membrane proteins may be isolated from an organism, such as Staphylococcus aureus, or made synthetically or by recombinant means.
- the protein may be synthesized by in vitro transcription translation.
- the amino acid sequence of the proteins may be modified to include non-naturally occurring amino acids or to increase the stability of the proteins. When the proteins are produced by synthetic means, such amino acids may be introduced during production.
- the proteins may also be modified following either synthetic or recombinant production.
- the proteins may also be produced using D-amino acids.
- the amino acids will be linked in reverse sequence in the C to N orientation. This is conventional in the art for producing such proteins.
- side chain modifications are known in the art and may be made to the side chains of the membrane proteins. Such modifications include, for example, modifications of amino acids by reductive alkylation by reaction with an aldehyde followed by reduction with NaBH4, amidination with methylacetimidate or acylation with acetic anhydride.
- Recombinant membrane proteins can be produced using standard methods known in the art. Nucleic acid sequences encoding a protein can be isolated and replicated using standard methods in the art. Nucleic acid sequences encoding a protein can be expressed in a bacterial host cell using standard techniques in the art. The protein can be introduced into a cell by in situ expression of the polypeptide from a recombinant expression vector. The expression vector optionally carries an inducible promoter to control the expression of the polypeptide.
- the apparatus 1 can be used for a wide range of applications.
- a membrane protein is inserted in the layer 11 .
- An electrical signal typically a current signal, developed between the electrode 21 in the recess 5 and the further electrode 24 in the chamber 7 is monitored, using the electrical circuit 26 .
- a voltage is also applied between the electrodes 21 and 24 , whilst monitoring the electrical signal.
- the form of the electrical signal, and in particular changes therein, provide information about the layer 11 and any membrane protein inserted therein.
- the apparatus 1 may be used to detect an analyte molecule that binds with an inserted membrane protein, or another stimulus, using stochastic sensing by detecting a change in the current flow indicating the presence of the analyte molecule or other stimulus. Similarly, the apparatus 1 may be used to detect the presence or absence of membrane pores or channels in a sample, by detecting a change in the current flow as the pore or channel inserts.
- the lipid bilayer may be used for a range of other purposes, such as studying the properties of molecules known to be present (e.g. DNA sequencing or drug screening), or separating components for a reaction.
- a first technique is, after application of the pre-treatment coating 30 to apply a voltage across the electrode 21 in the recess 5 and the further electrode 24 in the chamber 7 sufficient to reduce the amount of excess hydrophobic fluid covering the electrode 21 in the recess 5 . This is produces a similar effect to electro-wetting.
- FIGS. 10 a to 10 e This technique is illustrated in FIGS. 10 a to 10 e .
- the pre-treatment coating 30 is applied as shown in FIG. 10 a where the pre-treatment coating 30 covers the electrode 21 .
- aqueous solution 10 is flowed across the body 2 to cover the recess 5 so that aqueous solution 10 flows into the recess 5 .
- a voltage is applied which removes the pre-treatment coating 30 covering the electrode 21 , as shown in FIG. 10 c . This voltage will rupture any layer of amphiphilic molecules formed across the recess 5 . Therefore, next, as shown in FIG.
- aqueous solution 10 is flowed out of the chamber 7 to uncover the recess 5 .
- an amount of aqueous solution 10 will remain in the recess 5 .
- aqueous solution 10 having amphiphilic molecules added thereto, is flowed across the body 2 to re-cover the recess 5 so that the layer 11 of the amphiphilic molecules forms.
- the aqueous solution 10 flowed into the chamber 7 to re-covering the recess 5 could be different from the aqueous solution 10 flowed into the chamber 7 to first cover the recess 5 (in FIG. 10 b ) before applying the voltage.
- a second technique is to make an inner part of the internal surface of the recess 5 hydrophilic. This may be achieved by making the body 2 with two (or in general more) further layers 4 a and 4 b as shown in FIG. 11 , of which the innermost further layer 4 a (or layers) formed of a hydrophilic material, for example SiO 2 . Typically but without limitation, the innermost further layer 4 a might have a thickness of 2 ⁇ m.
- the outermost further layer 4 b (or layers) is formed of a hydrophobic material and as a result both of (a) the outermost surface of the body 2 around the recess and (b) the outer part of the internal surface of the recess 5 extending from the rim of the recess 5 is hydrophobic. This assists in the spreading of the pre-treatment coating. Indeed this property of these surfaces of the body 2 is desirable even if there is not an inner further layer 4 a formed of a hydrophilic material.
- outermost further layer 4 b might have a thickness of 1 ⁇ m, 3 ⁇ m, 5 ⁇ m, 10 ⁇ m, 20 ⁇ m or 30 ⁇ m.
- a third technique is to provide a hydrophillic surface on the electrode 21 which repels the applied pre-treatment coating 30 , whilst allowing ionic conduction from the aqueous solution 10 to the electrode 2 .
- This may be achieved by depositing a protective material on the electrode 21 .
- a range of protective materials may be used.
- One possibility is a conductive polymer, for example polypyrrole/polystyrene sulfonate as discussed above.
- Another possibility is a covalently attached hydrophilic species, such as thiol-PEG.
- the apparatus 1 described above has been made and used experimentally to demonstrate formation of a layer 11 , in particular being a lipid bilayer, and insertion of a membrane protein, in particular ⁇ -hemolysin. The following procedure was followed after manufacture of the apparatus 1 :
- step 1) the pre-treatment coating 30 was hexadecane dissolved in pentane.
- the quantity and volume of the pre-treatment coating 30 was varied for each test to obtain the optimum conditions for formation of the layer 11 .
- Insufficient pre-treatment coating 30 prevented formation of the layer 11 while excess pre-treatment coating 30 caused blocking of the recesses.
- routine variation of the amount allowed optimisation.
- the amphiphilic molecules were a lipid, in particular 1,2-diphytanoyl-sn-glycero-3-phosphocholine.
- the lipid was dissolved in pentane and then dried onto the surface of the cover 6 defining an internal surface of the chamber 7 before attaching the cover 6 on top of the body 2 .
- the aqueous solution 10 collected the lipid.
- Step 3 was performed by application of a large potential to across the electrodes 21 and 24 . This removed excess pre-treatment coating 30 from the electrode 21 . Although not required in every case, when performed this stage helped to condition the recess 5 for formation of the layer 11 and assisted subsequent measurement of electrical signals.
- the first conductive layer 20 was formed by a silver foil strips (25 ⁇ m thick, from Goodfellow) thermally laminated onto the substrate 3 using a 15 ⁇ m thick laminating film (Magicard) to form the further layer 4 .
- a circular recess 5 of diameter 100 ⁇ m was created further layer 4 using an excimer laser, exposing a circular silver electrode 21 of diameter 100 ⁇ m.
- the exposed silver was chloridised electrochemically as described previously.
- the second conductive layer 23 was a screen printing silver/silver chloride ink printed on the top side of the body 2 .
- the pre-treatment coating 30 comprising 0.5 ⁇ l of 1% heaxadecane +0.6 mg/ml DPhPC in pentane, was then applied to the body 2 and dried at room temperature.
- the cover 6 comprised a 1 mm thick silicon rubber body with a 250 ⁇ m thick Mylar lid. Lipid (4 ⁇ l of 10 mg/ml DPhPC in pentane) was applied to the inside of the cover 6 and allowed to dry at room temperature before attachment to the body 2 with self-adhesive.
- Addition of the aqueous solution 10 creates an “open circuit” connection between the electrodes, such that the current response to the applied potential waveform is large, typically saturating the current amplifier.
- a typical trace is shown in FIG. 16 , involving a current response greater than 20,000 pA to the 20 mV potential. This corresponds to a resistance of less than 1 M ⁇ , which is sufficiently small for use in conjunction with bilayer formation and pore current measurement.
- the aqueous solution 10 is removed from the chamber 7 and reintroduced.
- a layer 11 of the lipid collected from the internal surface of the chamber 7 is formed across the recess 5 .
- the formation is observed by an increase in the capacitive squarewave current response to just under 500 pA, for example as shown in FIG. 18 . This value is consistent with the capacitance expected for a circular lipid bilayer of diameter of order 100 ⁇ m and varies predictably for different geometries.
- FIG. 19 is a typical example with cyclodextrin present in the aqueous solution 10 and shows an expected current response with binding events confirming that the current is through the pores.
- the first conductive layer 20 was formed by etching the copper foil on an FR4 substrate typically used in printed circuit board manufacture.
- the board was then screen printed with a Ronascreen SPSRTM photoimageable solder mask to a depth of 25 ⁇ m and exposed to UV light on an Orbotech Paragon 9000 laser direct imaging machine and developed with KaCO 3 solution to create 100 ⁇ m circular apertures over the electrodes 21 .
- the pre-treatment coating 30 comprising 0.5 ⁇ l of 0.75% hexadecane in pentane, was then applied to the body 2 and dried at room temperature.
- the cover 6 comprised a 1 mm thick silicon rubber body with a 250 ⁇ m thick Mylar lid. Lipid (40 of 10 mg/ml DPhPC in pentane) was applied to the inside of the cover 6 and allowed to dry at room temperature before attachment to the body 2 with self-adhesive.
- FIG. 22 shows a typical current trace showing cyclodextrin binding events with wild-type ⁇ -hemolysin pores.
- the apparatus 1 has a single chamber 7 , but creates the layer 11 in situ during the test and captures a reservoir of electrolyte in the recess 5 under the layer 11 which allows continuous stable measurement of current passing through protein pores inserted in the layer 11 .
- the layer 11 formed is of high quality and is localised to the area of the recess 5 , ideal for high-fidelity current measurements using membrane protein pores.
- Apparatuses having an array of recesses 5 have been tested and demonstrated successful formation of an array of layers 11 , showing the possibility of creating a miniaturised array of close packed individually addressable layers recording current signals in parallel from a test sample.
- an apparatus 1 having an array of recesses 5 can be formed simply using the manufacturing techniques described above but instead forming plural recesses 5 .
- the first conductive layer 20 is divided to form a separate electrode 21 , contact 22 and intermediate conductive track 27 in respect of each recess 5 .
- the apparatus 1 has a single chamber 7 with a single electrode 24 common to all the recesses 5 .
- FIGS. 23 to 25 show first to third designs in which the apparatus 1 is modified by providing, respectively, four, nine and 128 recesses 5 in the further layer 4 .
- the first conductive layer 20 is divided, as shown, respectively, in FIGS. 26 to 28 being plan views of the substrate 3 .
- the first conductive layer 20 provides, in respect of each recess 5 : an electrode 21 underneath the recess 5 ; a contact 22 exposed for connection of the external circuit 26 and a track 27 between the electrode 21 and the contact 22 .
- each electrode 21 , and its associated track 27 and contact 22 is electrically insulated from each other allowing separate measurement of current signals from each recess 5 .
- Manufacture of the apparatus 1 may be performed using the techniques described above using lamination of polymer films or photolithography using silicon wafers.
- Apparatuses 1 having plural recesses 5 have been made and used experimentally to demonstrate formation of a layer 11 , in particular being a lipid bilayer, and insertion of a membrane protein, in particular ⁇ -hemolysin.
- the experimental procedure was as described above for an apparatus 1 having a single recess 5 , except that formation of the layer 5 and membrane protein insertion was observed at plural recesses 5 .
- An apparatus of the first design having four recesses 5 was manufactured by the technique described above of lamination onto a polymer substrate 3 .
- the first conductive layer 20 was silver vapour deposited on a polyester sheet substrate 3 .
- the further layer 4 was a 15 ⁇ m thick laminating film thermally laminated on top.
- the four recesses 5 of 100 ⁇ m diameter were formed at a pitch of 300 ⁇ m by an excimer laser.
- An apparatus of the second design having nine recesses 5 was manufactured by the technique described above of photolithography using silicon wafer substrates 2 .
- the further layer 4 was 5 ⁇ m thick SU8 photoresist.
- the nine circular recesses 5 were formed at a pitch of 300 ⁇ m by photolithography.
- the recesses 9 had different diameters, in particular of 5 ⁇ m, 10 ⁇ m, 15 ⁇ m, 20 ⁇ m, 20 ⁇ m, 30 ⁇ m, 40 ⁇ m, 50 ⁇ m, and 100 ⁇ m.
- the substrate 3 was bonded to a printed circuit board with separate tracks connected to each contact 22 and 25 . Epoxy was added across the contacts 22 and 25 for protection
- a multichannel electrical circuit 26 was created with corresponding software. Testing was computer automated using a syringe pump to provide fluidics control of the repeated application and removal of the aqueous solution 10 .
- FIG. 30 typical current traces for recesses 5 constructed with gold electrodes and operating without a redox couple in solution are shown in FIG. 30 demonstrating simultaneous formation of eight layers 11 , each having one or two ⁇ -hemolysin pores inserted, with cyclodextrin binding events. Again there is no cross-talk and this confirms that the layers 11 are operating independently and can produce meaningful measurements in parallel.
- the apparatus 1 demonstrates successful formation of a layer 11 across the recess 5 of each diameter in the range of 5 ⁇ m to 100 ⁇ m. Accordingly the apparatus 1 was used to investigate the role of the diameter of the recess 5 and the quantity of pre-treatment coating applied, by experimentally testing the percentage success rate of forming a layer 5 with three different concentrations of pre-treatment coating 30 , namely 0.5%, 1.0%, and 2.0% hexadecane in pentane. The results showed that in the case of too little pretreatment coating 30 , it was not possible to form the layer 11 across the range of diameters of recess 5 . Furthermore in the case of too much pretreatment coating 30 , it was not possible to wet the electrode 21 and formation of the layer 11 could not be observed.
- the yield of formation of layers 11 was greater than 60% for the range of diameters 15 ⁇ m to 100 ⁇ m.
- Factors affecting layer formation include, but are not limited to, pretreatment coating 30 , diameter of recess 5 , depth of recess 5 , aspect ratio of recess 5 , surface properties of the recess 5 , surface properties of the surfaces around the recess, fluid flow within the chamber 7 , the amphiphilic molecules used in the layer formation and the physical and electrical properties of the electrode 21 within the recess 5 .
- Subsequent experiments have demonstrated yield of formation of layers 11 , verified by stochastic binding signals of inserted membrane channels, greater than 70% using the 128 recesses, each 100 ⁇ m in diameter, of the device of FIG. 28 .
- the conductive tracks 27 from the electrode 21 to the contact 22 is formed on a surface of the substrate 3 under the further layer. This may be referred to as a planar escape route for the conductive track 27 .
- the separate conductive tracks 27 allow each electrode 21 to be connected individually to a dedicated low-noise high-input impedance picoammeter in the circuit 26 whilst minimising the signal deterioration due to noise and bandwidth reduction.
- planar conductive tracks 27 are ideal for an apparatus 1 having a small number of recesses 5 and a thick layer between the tracks 27 and the aqueous solution 10 .
- the electrical connection between the electrodes 21 and the amplifier circuit desirably has low parasitic capacitance and low leakage to the surroundings.
- Parasitic capacitance causes noise and hence signal deterioration and bandwidth reduction. Leakage also increases noise, as well as introducing an offset current.
- the conductive tracks 27 experience some degree of parasitic capacitance and leakage, both between tracks 27 and between track and aqueous solution 10 .
- the number of recesses in the array increases, the number of electrical connections to escape increases and with a planar escape route, a practical limit is reached where the density of the conductive tracks 27 creates too much parasitic capacitance and/or leakage between tracks.
- the thickness of the layer 4 decreases the capacitance and/or leakage between the tracks 27 and the aqueous solution 10 increases.
- typical figures may be obtained by modelling the lipid bilayer as a capacitive element with a typical value for the capacitance per unit area of 0.8 ⁇ F/cm 2 .
- the parasitic capacitance between track 27 and aqueous solution 10 can be crudely modelled as a capacitative element with the area of track 27 exposed, through the layer, to the aqueous solution.
- Typical values for the track 27 may be 50 ⁇ m wide with 2 mm exposed and a relative permittivity (dielectric constant) of the layer around 3 .
- the capacitance is 63 pF with a track-solution parasitic capacitance of 0.13 pF.
- scaling to smaller bilayers of 5 ⁇ m diameter and 1 ⁇ m deep the capacitance is 0.16 pF with parasitic capacitance 0.53 pF.
- the parasitic capacitance dominates.
- a modification shown in FIG. 31 is to replace the conductive track 27 by a conductive path 28 which extends through the body 2 to a contact 29 on the opposite side of the body 2 from the electrode 21 .
- the conductive path 28 extends through the substrate 3 .
- this substrate 3 provides a thicker dielectric between the conductive paths 28 than is possible between the planar conductive paths 27 , a much lower parasitic capacitance is achieved.
- the leakage is low due to the thickness and dielectric properties of the substrate 3 . Consequently, the use of the conductive paths 28 effectively increases the number of recesses 5 which may be accomodated in the body 2 before the practical limits imposed by parasitic capacitance and/or leakage are met.
- This form of interconnect can be attached to a low-capacitance multi-layer substrate 61 , which allows a far greater number of electrical escape routes by virtue of the number of layers and the low dielectric constant of the material.
- solder bump technology also known as “flip chip” technology
- a suitable connector allows the apparatus 1 shown in FIG. 31 , excluding the substrate 61 , to be made as low cost disposable part.
- the conductive path 28 may be formed using known through-wafer interconnection technology.
- Types of through-wafer interconnects which may be applied to form the conductive path include without limitation:
- through-wafer interconnects formed by producing a via through the silicon wafer, isolating the internal surface of via and filling the via with a conducting material, or alternatively the conductive path 28 is formed by producing a semiconductor PN junction in the form of a cylindrical via through the silicon substrate;
- through-wafer interconnects formed by methods including laser drilling, wet etching and filling vias with metal or doped semiconductor material;
- substrates 3 made of polymers through-wafer interconnects formed by methods including laser drilling, laser ablation, screen printed conductors and known printed circuit board techniques.
- FIG. 31 illustrates the use of solder bump connections.
- deposited on each contact 29 are respective solder bumps 60 on which a circuit element 61 is mounted so that the solder bumps 60 make electrical contact with a track 62 on the circuit element 61 .
- the circuit element 61 may be a printed circuit board for example as shown in FIG. 13 .
- the circuit element 61 could be an integrated circuit chip or a laminate, for example a low temperature cured ceramic package. Such an integrated circuit chip or laminate may be used as a method of spreading out connections, connecting to a further solder bump array on the opposite side of the integrated circuit chip or laminate with a greater pitch.
- FIG. 32 An example of this is shown in which the circuit element 61 is an integrated circuit chip or a laminate providing connections from the solder bumps 60 deposited on the body 2 to further solder bumps 63 arrayed at a greater pitch and used to connect to a further circuit element 64 , for example a printed circuit board.
- the circuit element 61 being an integrated circuit chip or laminate may also be used to escape connections sideways in a multi-layer format.
- MIS Metal-Insulator-Semiconductor
- PN junction type of through-wafer interconnect is a semiconductor junction formed into a cylindrical via through a silicon chip.
- Each type of through-wafer interconnection is formed on silicon wafers that have been thinned down to less than 0.3 mm to save DRIE processing time in making the holes.
- the important feature of PN junction type through-wafer interconnects is the low capacitance provided by having a large depletion region compared to the MIS type of interconnect. This is partially helped by increasing the reverse-bias of the junction.
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Abstract
To form a layer separating two volumes of aqueous solution, there is used an apparatus comprising elements defining a chamber, the elements including a body of non-conductive material having formed therein at least one recess opening into the chamber, the recess containing an electrode. A pre-treatment coating of a hydrophobic fluid is applied to the body across the recess. Aqueous solution, having amphiphilic molecules added thereto, is flowed across the body to cover the recess so that aqueous solution is introduced into the recess from the chamber and a layer of the amphiphilic molecules forms across the recess separating a volume of aqueous solution introduced into the recess from the remaining volume of aqueous solution.
Description
- In one aspect, the present invention relates to the formation of layers of amphiphilic molecules such as lipid bilayers. It is particularly concerned with the formation of high quality layers suitable for applications requiring measurement of electrical signals with a high degree of sensitivity, for example single channel recordings and stochastic sensing for biosensor or drug screening applications. In one particular aspect, it is concerned with applications employing arrays of layers of amphiphilic molecules, for example lipid bilayers. In another aspect, the present invention relates to the performance of an electrode provided in a recess, for example for conducting electro-physiological measurements.
- The potential for using cellular proteins for biosensing and drug discovery applications has long been appreciated. However there are many technical challenges to overcome in developing this technology to fully realise the potential. There is a wealth of literature on using fluorescent and optical approaches, but the focus of this document is on the measurement of electrical signals to recognise analytes in biosensing.
- In one type of technique, a layer of amphiphilic molecules may be used as the layer separating two volumes of aqueous solution. The layer resists the flow of current between the volumes. A membrane protein is inserted into the layer to selectively allow the passage of ions across the layer, which is recorded as an electrical signal detected by electrodes in the two volumes of aqueous solution. The presence of a target analyte modulates the flow of ions and is detected by observing the resultant variations in the electrical signal. Such techniques therefore allow the layer to be used as a biosensor to detect the analyte. The layer is an essential component of the single molecule biosensor presented and its purpose is two-fold. Firstly the layer provides a platform for the protein which acts as a sensing element. Secondly the layer isolates the flow of ions between the volumes, the electrical resistance of the layer ensuring that the dominant contribution of ionic flow in the system is through the membrane protein of interest, with negligible flow through the bilayer, thus allowing detection of single protein channels.
- A specific application is stochastic sensing, where the number of membrane proteins is kept small, typically between 1 and 100, so that the behaviour of a single protein molecule can be monitored. This method gives information on each specific molecular interaction and hence gives richer information than a bulk measurement. However, due to the small currents involved, typically a few pA, requirements of this approach are a very high resistance seal, typically at least 1 GΩ and for some applications one or two orders of magnitude higher, and sufficient electrical sensitivity to measure the currents. While the requirements for stochastic sensing have been met in the laboratory, the conditions and expertise required limit its use. In addition, the laboratory methods are laborious and time-consuming and are not easily scalable to high-density arrays, which are desirable for any commercial biosensor. Furthermore, the fragility of single bilayer membranes means that anti-vibration tables are often employed in the laboratory.
- By way of background, existing techniques for forming layers of amphiphilic molecules such as lipid bilayers will be reviewed.
- Several methods for forming planar artificial lipid bilayers are known in the art, most notably including folded bilayer formation (e.g. Montal & Mueller method), tip-dipping, painting, patch clamping, and water-in-oil droplet interfaces.
- At present, the bulk of routine single ion channel characterisation in research labs is performed using folded bilayers, painted bilayers or tip-dip methods. These methods are used either for the ease of bilayer formation, or for the high resistive seals that can be formed (eg 10-100 GΩ). Tip-dip bilayers and bilayers from patch-clamping of giant unilamellar liposomes are also studied as they can be formed in a solvent free manner, which is thought to be important for the activity of some protein channels.
- The method of Montal & Mueller (Proc. Natl. Acad. Sci. USA. (1972), 69, 3561-3566) is popular as a cost-effective and relatively straightforward method of forming good quality folded lipid bilayers suitable for protein pore insertion, in which a lipid monolayer is carried on the water/air interface past either side of an aperture in a membrane which is perpendicular to that interface. Typically, the lipid is added to the surface of the aqueous electrolyte solution by first dissolving it in an organic solvent, a drop of which is then allowed to evaporate on the surface of the aqueous solution on either side of the aperture. Once the organic solvent has been evaporated, the solution/air interfaces are physically moved up and down past either side of the aperture until a bilayer is formed. The technique requires the presence of a hydrophobic oil applied as a pre-treatment coating to the aperture surface. The primary function of the hydrophobic oil is to form an annulus region between the bilayer and the aperture film where the lipid monolayers must come together over a distance typically between 1 and 25 μm.
- Tip-dipping bilayer formation entails touching the aperture surface (e.g. a pipette tip) onto the surface of a test solution that is carrying a monolayer of lipid. Again the lipid monolayer is first generated at the solution/air interface by evaporating a drop of lipid dissolved in organic solvent applied to the solution surface. The bilayer is then formed by mechanical actuation to move the aperture into/out of the solution surface.
- For painted bilayers, the drop of lipid dissolved in organic solvent is applied directly to the aperture, which is submerged in the aqueous test solution. The lipid solution is spread thinly over the aperture using a paint brush or equivalent. Thinning of the solvent results in formation of a lipid bilayer, however, complete removal of the solvent from the bilayer is difficult and consequently the bilayer formed is less stable and more noise prone during measurement.
- Patch-clamping is commonly used in the study of biological cell membranes, whereby the cell membrane is clamped to the end of a pipette by suction and a patch of the membrane becomes attached over the aperture. The method has been adapted for artificial bilayer studies by clamping liposomes which then burst to leave a lipid bilayer sealing over the aperture of the pipette. This requires stable giant unilamellar liposomes and the fabrication of small apertures in glass surfaced materials.
- Water-in-oil droplet interfaces are a more recent invention in which two aqueous samples are submerged in a reservoir of hydrocarbon oil containing lipid. The lipid accumulates in a monolayer at the oil/water interface such that when the two samples are brought into contact a bilayer is formed at the interface between them.
- In any of these techniques, once the bilayer has been formed, the protein is then introduced to the bilayer either by random collision from the aqueous solution, by fusion of vesicles containing the protein, or by mechanically transporting it to the bilayer, for example on the end of a probe device such as an agar tipped rod.
- There have been great efforts recently to increase the ease of bilayer formation using micro fabrication. Some techniques have attempted essentially to miniaturise standard systems for folded lipid bilayers. Other techniques include bilayer formation on solid substrates or directly on electrode surfaces, through either covalent attachment or physical adsorption.
- A large proportion of the devices that are capable of performing stochastic sensing form a bilayer by using a variant of the folded lipid bilayers technique or the painted bilayer technique. To date most have concentrated either on novel methods of aperture formation or on utilising the emerging technologies in micro fabrication to miniaturise the device or to create a plurality of addressable sensors.
- An example is Suzuki et al., “Planar lipid bilayer reconstitution with a micro-fluidic system”, Lab Chip, (4), 502-505, 2004. Herein, an aperture array is created by etching a silicon substrate, followed by a surface treatment to encourage the bilayer formation process, although the disclosed rate of successful bilayer formation is very low (two out of ten).
- A more recent example is disclosed in Sandison, et al., “Air exposure technique for the formation of artificial lipid bilayers in microsystems”, Langmuir, (23), 8277-8284, 2007. Herein the device fabricated from poly(methylmethacrylate) contains two distinct aqueous chambers. Problems with the reproducibility of bilayer formation are attributed to the difficulty in removing the excess hydrophobic material from the aperture, and tackled by using a period of air exposure to aid the bilayer formation process to thin the pre-treatment.
- The devices of both Sandison et al. and Suzuki et al. are both miniaturised versions of a standard painted bilayer technique with two distinct fluidic chambers separated by a septum containing an aperture across which the bilayer is formed, one chamber being filled before the other. This presents a number of difficulties for scaling up the system to a large number of individually addressable bilayers, as at least one of the aqueous chambers must be a distinct chamber with no electrical or ionic connectivity to any other chamber. Sandison et al. created a device with three fluid chambers, each with separate fluidics, an approach which would be difficult to scale to large numbers of bilayers. Suzuki et al. tried to address this problem by using a hydrophobic photoresist layer to create small aqueous chambers on top of the aperture containing substrate. In this case, it is difficult to control the flow of solution across the aperture containing interface and the use of small volumes exposed to air makes the apparatus susceptible to evaporation effects. In both cited examples, the need for the individual aqueous chambers for each bilayer means that a large sample volume must be used to fill all the chambers.
- An example of biosensor device using a supported lipid bilayer is disclosed in U.S. Pat. No. 5,234,566. The device is capacitive. A gated ion channel responds to an analyte, the binding of this analyte causes a change in the gating behaviour of the ion channel, and this is measured via the electrical response of the membrane capacitance. To support the lipid bilayer, there is used a monolayer of alkane-thiol molecules on a gold electrode, which provides a scaffold for a lipid monolayer to self-assemble onto. This monolayer can incorporate ion channels such as gramicidin which are used as the sensing element of the device. Variations on this method have been used to create a tethered lipid bilayer onto an electrode surface to incorporate other membrane proteins. However, the approach has a number of drawbacks, the first is that the small aqueous volume present under the lipid bilayer, typically of the order of 1 nm to 10 nm thick, does not contain enough ions to perform a direct current measurement for any useful period of time. This is an effect common to nearly all tethered bilayer systems on solid supports. For recordings of any meaningful duration, an alternating current measurement must be used to overcome the ionic depletion at the electrode, but that limits the sensitivity of the device.
- An example of a biosensor device using a supported lipid bilayer is disclosed in Urisu et al., “Formation of high-resistance supported lipid bilayer on the surface of a silicon substrate with microelectrodes”, Nanomedicine, 2005, (1), 317-322. This device exploits the strong surface adhesion between phospholipid molecules and a SiO2 surface to form a supported bilayer. A silicon oxide surface is modified, using etching techniques common in silicon chip production, to expose small channels to an electrode surface. A bilayer is then formed on the silicon oxide surface, resulting in an electrical resistance of a few MΩ. In this system, the wells created by this process could not be individually addressed.
- In both of the cited examples using a supported lipid bilayer, it is very difficult to form a high resistive seal using these methods. Although the resistance may be sufficient to observe a change arising from a large number of ion channels, single channel or stochastic measurements, which are inherently more sensitive, are incredibly challenging using this methodology.
- There are a number of problems with the supported bilayer approach in these documents and in general, which makes this system unsuitable. The first problem lies with the resistance of the bilayer membrane which is typically about 100 MΩ. While this may be suitable for examining protein behaviour at large protein concentrations, it is not sufficient for a high-fidelity assay based on single molecule sensing, typically requiring a resistance of at least 1 GΩ and for some applications one or two orders of magnitude higher. The second problem is the small volume of solution trapped in the short distance between the bilayer and the solid support, typically of the order of 1 nm. This small volume does not contain many ions, affecting the stability of the potential across the bilayer and limiting the duration of the recording.
- A number of methods have been proposed to overcome the problems with solid supported bilayers. One option is to incorporate a chemical linkage between the bilayer and the surface, either a small polyethylene glycol layer is introduced (polymer cushioned bilayers), or the lipid is chemically modified to contain a small hydrophilic linkage and reacted with the surface providing a scaffold for vesicle deposition (tethered bilayers). While these methods have increased the ionic reservoir beneath the lipid bilayer, they are inconvenient to implement and have done little to decrease the current leakage across the bilayer.
- The techniques used in the silicon chip industry provide an attractive technology for creating a large number of electrodes that could be used in biosensor applications. This approach is disclosed in the related applications U.S. Pat. No. 7,144,486 and U.S. Pat. No. 7,169,272. US-7,144,486 discloses a method of fabricating a microelectrode device containing microcavities etched into layers of insulator material. The devices are said to have a wide range of electrochemical applications in which electrodes in the cavities measure electrical signals. It is stated that thin films may be suspended across the cavities. Several types of film are mentioned, including being a lipid bilayer. However this is merely a proposal and there is no disclosure of any technique for forming the lipid bilayer, nor any experimental report of this. Indeed the related application U.S. Pat. No. 7,169,272, which does report experimental formation of lipid bilayers in the same type of device, discloses the supported lipid bilayers being chemically attached directly on the electrodes. This uses similar techniques to those presented in Osman et al. cited above and suffers from the same drawbacks relating to the lack of a sufficiently high resistive seal for stochastic measurements and the lack of an ionic reservoir for recording ionic flow across the bilayer system.
- To summarise, the known technologies summarised above either present methods of bilayer formation which can not reproducibly achieve high resistance, or suffer from low ionic reservoirs and are not capable of high duration direct current measurements, or require a separate fluidic chamber for each array element, limiting the scale up of that device to a high-density array. It would be desirable to reduce these problems.
- According to a first aspect of the present invention, there is provided a method of forming a layer separating two volumes of aqueous solution, the method comprising:
- (a) providing an apparatus comprising elements defining a chamber, the elements including a body of non-conductive material having formed therein at least one recess opening into the chamber, the recess containing an electrode;
- (b) applying a pre-treatment coating of a hydrophobic fluid to the body across the recess;
- (c) flowing aqueous solution, having amphiphilic molecules added thereto, across the body to cover the recess so that aqueous solution is introduced into the recess from the chamber and so that a layer of the amphiphilic molecules forms across the recess separating a volume of aqueous solution introduced into the recess from the remaining volume of aqueous solution.
- Such a method allows the formation of layers of amphiphilic molecules which are of sufficiently high quality for sensitive techniques such as stochastic sensing whilst using apparatus and techniques which are straightforward to implement.
- The apparatus used is relatively simple, involving most importantly a body of ionically non-conductive material having formed therein at least one recess. It has been demonstrated, surprisingly, that it is possible to form a layer of the amphiphilic molecules across such a recess simply by flowing the aqueous solution across the body to cover the recess. To achieve this a pre-treatment coating of a hydrophobic fluid is applied to the body across the recess. The pre-treatment coating assists formation of the layer. The layer is formed without any need for a complicated apparatus involving two chambers separated by a septum and requiring a complicated fluidics arrangement to achieve separate filling. This is because the method does not require the recess to be pre-filled prior to introducing aqueous solution into the chamber above. Instead, the aqueous solution is introduced into the recess from the chamber. Despite this, it is still possible to form the layer by mere control of the aqueous solution flowing into the chamber. Such flow control is a straightforward practical technique.
- Importantly, the method allows the formation of layers of amphiphilic molecules which are suitable for high sensitivity biosensor applications such as stochastic sensing and single channel recording. It has been demonstrated possible to form layers of high resistance providing highly resistive electrical seals, having an electrical resistance of 1 GΩ or more, typically at least 100 GΩ. which, for example, enable high-fidelity stochastic recordings from single protein pores. This is achieved whilst trapping a volume of aqueous solution in the recess between the layer and the electrode. This maintains a significant supply of electrolyte. For example, the volume of aqueous solution is sufficient to allow stable continuous dc current measurement through membrane proteins inserted in the layer. This contrasts significantly with the known techniques described above using supported lipid bilayers.
- Furthermore, the simple construction of the apparatus allows the formation of a miniaturised apparatus having an array of plural recesses and allowing the layer across each recess to be electrically isolated and individually addressed using its own electrode, such that the miniaturised array is equivalent to many individual sensors measuring in parallel from a test sample. The recesses may be relatively densely packed, allowing a large number of layers to be used for a given volume of test sample. Individual addressing may be achieved by providing separate contacts to each electrode which is simple using modern microfabrication techniques, for example lithography.
- Furthermore, the method allows the formation of multiple layers of the amphiphilic molecules within a single apparatus across the plural recesses in an array using a very straightforward technique.
- In most applications, one or more membrane proteins is subsequently inserted into the layer. Certain membrane proteins that can be used in accordance with the invention are discussed in more detail below.
- According to further aspects of the invention, there is provided an apparatus suitable for implementing such methods of formation of a layer of amphiphilic molecules.
- Further details and preferred features of the invention will now be described.
- The amphiphilic molecules are typically a lipid. In this case the layer is a bilayer formed from two opposing monolayers of lipid. The lipids can comprise one or more lipids. The lipid bilayer can also contain additives that affect the properties of the bilayer. Certain lipids and other amphiphilic molecules, and additives that can be used in accordance with the invention are discussed in more detail below.
- Various techniques may be applied to add the amphiphilic molecules to the aqueous solution.
- A first technique is simply to add the amphiphilic molecules to the aqueous solution outside the apparatus before introducing the aqueous solution into the chamber.
- A second technique which has particular advantage is, before introducing the aqueous solution into the chamber, to deposit the amphiphilic molecules on an internal surface of the chamber, or elsewhere in the flow path of the aqueous solution, for example in a fluidic inlet pipe connected to the inlet. In this case, the aqueous solution covers the internal surface during step (c) whereby the amphiphilic molecules are added to the aqueous solution. In this manner the aqueous solution is used to collect the amphiphilic molecules from the internal surface. Such deposition of the amphiphilic molecules has several advantages. It allows the formation of layer of amphiphilic molecules in the absence of large amounts of organic solvent, as would typically be present if the amphiphilic molecules were added directly to the aqueous solution. This means that it is not necessary to wait for evaporation of the organic solvent before the layer can be formed. In addition, this means that the apparatus is not required to be made from materials that are insensitive to organic solvents. For instance, organic-based adhesives can be used and screen-printed conductive silver/silver chloride paste can be used to construct electrodes.
- Advantageously, the deposited amphiphilic molecules can be dried. In this case, the aqueous solution is used to rehydrate the amphiphilic molecules. This allows the amphiphilic molecules to be stably stored in the apparatus before use. It also avoids the need for wet storage of amphiphilic molecules. Such dry storage of amphiphilic molecules increases shelf life of the apparatus.
- Several techniques may be used to insert a membrane protein into the layer of amphiphilic molecules.
- A first technique is simply for the aqueous solution to have a membrane protein added thereto, whereby the membrane protein is inserted spontaneously into the layer of amphiphilic molecules. The membrane protein may be added to the aqueous solution outside the apparatus before introducing the aqueous solution into the chamber. Alternatively the membrane protein may be deposited on an internal surface of the chamber before introducing the aqueous solution into the chamber. In this case, the aqueous solution covers the internal surface during step (c), whereby the membrane protein is added to the aqueous solution.
- A second technique is for the aqueous solution to have vesicles containing the membrane protein added thereto, whereby the membrane protein is inserted on fusion of the vesicles with the layer of amphiphilic molecules.
- A third technique is to insert the membrane protein by carrying the membrane protein to the layer on a probe, for example an agar-tipped rod.
- To form the layer of amphiphilic molecules, the aqueous solution is flowed across the body to cover the recess. Formation is improved if a multi-pass technique is applied in which aqueous solution covers and uncovers the recess at least once before covering the recess for a final time. This is thought to be because at least some aqueous solution is left in the recess which assists formation of the layer in a subsequent pass.
- The pre-treatment coating is a hydrophobic fluid which assists formation of the layer by increasing the affinity of the amphiphilic molecules to the surface of the body around the recess. In general any pre-treatment that modifies the surface of the surfaces surrounding the aperture to increase its affinity to lipids may be used. Certain materials for the pre-treatment coating that can be used in accordance with the invention are discussed in more detail below.
- To assist in the spreading of the pre-treatment coating, surfaces including either or preferably both of (a) the outermost surface of the body around the recess and (b) at least an outer part of the internal surface of the recess extending from the rim of the recess may be hydrophobic. This may be achieved by making the body with an outermost layer formed of a hydrophobic material.
- Another way to achieve this is for the surfaces to be treated by a fluorine species, such as a fluorine radical, for example by treatment with a fluorine plasma during manufacture of the apparatus.
- The application of the pre-treatment coating may leave excess hydrophobic fluid covering said electrode contained in the recess. This potentially insulates the electrode by reducing ionic flow, thereby reducing the sensitivity of the apparatus in measuring electrical signals. However various different techniques may be applied to minimise this problem.
- A first technique is to apply a voltage across the electrode in the recess and a further electrode in the chamber sufficient to reduce the amount of excess hydrophobic fluid covering said electrode contained in the recess. This produces a similar effect to electro-wetting. The voltage is applied after flowing aqueous solution across the body to cover the recess so that aqueous solution flows into the recess. As the voltage will rupture any layer formed across the recess, subsequently the aqueous solution is flowed to uncover the recess, and then aqueous solution, having amphiphilic molecules added thereto, is flowed across the body to re-cover the recess so that a layer of the amphiphilic molecules forms across the recess.
- A second technique is to make an inner part of the internal surface of the recess hydrophilic. Typically this will be applied in combination with making the outer part of the internal surface of the recess hydrophobic. This may be achieved by making the body with an inner layer formed of a hydrophilic material and an outermost layer formed of a hydrophobic material.
- A third technique is to provide on the electrode a hydrophillic surface, for example a protective material, which repels the hydrophobic fluid applied in step (c) whilst allowing ionic conduction from the aqueous solution to the electrode. The protective material may be a conductive polymer, for example polypyrrole/polystyrene sulfonate. Alternatively, the protective material may be a covalently attached hydrophilic species, such as thiol-PEG.
- In general, a wide range of constructional features may be employed in the apparatus to form the body of non-conductive material, the at least one recess formed therein and the other elements defining the chamber. Examples are described in further detail below.
- According to a second aspect of the present invention, there is provided a method of improving the performance of an electrode in a recess in conducting electro-physiological measurements, the method comprising depositing a conductive polymer on the electrode.
- Further according to a second aspect of the present invention, there is provided an apparatus for conducting electro-physiological measurements, the apparatus comprising, a body having a recess in which an electrode is located, wherein a conductive polymer is provided on the electrode.
- It has been discovered that the providing a conductive polymer on an electrode in a recess can improve the performance of the electrode in conducting electro-physiological measurements. One advantage is to improve the electrode's performance as a stable electrode for conducting electro-physiological measurements. A further advantage is to increase the charge reservoir available to the electrode within the recess without increasing the volume of aqueous solution contained in the recess.
- To allow better understanding, an embodiment of the present invention will now be described by way of non-limitative example with reference to the accompanying drawings, in which:
-
FIG. 1 is a perspective view of an apparatus; -
FIG. 2 is a cross-sectional view of the apparatus ofFIG. 1 , taken along line II-II inFIG. 1 , and showing the introduction of an aqueous solution; -
FIG. 3 is a cross-sectional view of the apparatus, similar to that ofFIG. 2 but showing the apparatus full of aqueous solution; -
FIG. 4 is sequence of a cross-sectional, partial views of the recess in the apparatus over an electrochemical electrode modification process; -
FIG. 5 is an SEM image of a recess formed by CO2 laser drilling; -
FIG. 6 is an OM image of a recess formed using photolithography; -
FIGS. 7 a and 7 b are 3D and 2D LP profiles, respectively, of a recess formed using photolithography; -
FIGS. 8 a and 8 b are 3D and 2D LP profiles, respectively, of a recess formed using photolithography, after electoplating; -
FIG. 9 is a cross-sectional, partial view of the recess in the apparatus with a pre-treatment coating applied; -
FIGS. 10 a to 10 e are a sequence of cross-sectional, partial view of the recess in the apparatus during a method of removing excess pre-treatment coating; -
FIG. 11 is a cross-sectional, partial view of the recess in the apparatus having plural further layers in the body; -
FIG. 12 is a diagram of an electrical circuit; -
FIG. 13 is a perspective view of the apparatus and electrical circuit mounted on a printed circuit board; -
FIG. 14 is a diagram of an electrical circuit for acquiring plural signals in parallel; -
FIG. 15 is a graph of the applied potential and current response for a dry apparatus; -
FIG. 16 is a graph of the applied potential and current response for a wet apparatus; -
FIG. 17 is a graph of the applied potential and current response on electro-wetting of the apparatus; -
FIG. 18 is a graph of the applied potential and current response on formation of a layer of amphiphilic molecules; -
FIGS. 19 to 22 are graphs of the applied potential and current response for various different apparatuses; -
FIGS. 23 to 25 are plan views of a further layer in a modified apparatus having plural recesses; -
FIGS. 26 to 28 are plan views of the substrate in the modified apparatuses having plural recesses; -
FIGS. 29 and 30 are graphs of the current response for two different apparatuses having plural recesses; -
FIG. 31 is a cross-sectional view of a portion of a modified apparatus; -
FIG. 32 is a cross-sectional view of another modified apparatus; -
FIG. 33 is a flow chart of a method of manufacture of the apparatus; -
FIGS. 34 a and 34 b are 3D and 2D surface profiles of a recess having an electrode modified by electropolymerisation of polypyrrole, measured by profilometry; -
FIG. 35 is a graph of current recorded on an array of recesses having an electrode modified by electropolymerisation of polypyrrole. - An
apparatus 1 which may be used to form a layer of amphiphilic molecules is shown inFIG. 1 . - The
apparatus 1 includes abody 2 having layered construction as shown inFIGS. 2 and 3 comprising asubstrate 3 of non-conductive material supporting afurther layer 4 also of non-conductive material. In the general case, there may be pluralfurther layers 4, as described further below. - A
recess 5 is formed in thefurther layer 4, in particular as an aperture which extends through thefurther layer 4 to thesubstrate 3. In the general case, there may beplural recesses 5, as described further below. - The
apparatus 1 further includes acover 6 which extends over thebody 2. Thecover 6 is hollow and defines achamber 7 which is closed except for aninlet 8 and anoutlet 9 each formed by openings through thecover 6. The lowermost wall of thechamber 7 is formed by thefurther layer 4 inFIG. 2 , but as an alternative thefurther layer 4 could be shaped to provide side walls. - As described further below, in use
aqueous solution 10 is introduced into thechamber 7 and alayer 11 of amphiphilic molecules is formed across therecess 5 separatingaqueous solution 10 in therecess 5 from the remaining volume of aqueous solution in thechamber 7. The apparatus includes the following electrode arrangement to allow measurement of electrical signals across thelayer 11 of amphiphilic molecules. - Use of a
chamber 7 which is closed makes it very easy to flowaqueous solution 10 into and out of thechamber 7. This is done simply by flowing theaqueous solution 10 through theinlet 8 as shown inFIG. 2 until thechamber 7 is full as shown inFIG. 3 . During this process, gas (typically air) in thechamber 7 is displaced by theaqueous solution 10 and vented through theoutlet 9. For example, a simple fluidics system attached to theinlet 8 may be used. This may be as simple as a plunger, although more complicated systems may be used to improve the control. However, thechamber 7 is not necessarily closed and may be open, for example by forming thebody 2 as a cup. - The
substrate 3 has a firstconductive layer 20 deposited on the upper surface of thesubstrate 3 and extending under thefurther layer 4 to therecess 5. The portion of the firstconductive layer 20 underneath therecess 5 constitutes anelectrode 21 which also forms the lowermost surface of therecess 5. The firstconductive layer 20 extends outside thefurther layer 4 so that a portion of the firstconductive layer 20 is exposed and constitutes acontact 22. - The
further layer 4 has a secondconductive layer 23 deposited thereon and extending under thecover 6 into thechamber 7, the portion of the secondconductive layer 23 inside thechamber 7 constituting anelectrode 24. The secondconductive layer 23 extends outside thecover 6 so that a portion of the secondconductive layer 23 is exposed and constitutes acontact 25. - The
electrodes recess 5 andchamber 7. This allows measurement of electrical signals across thelayer 11 of amphiphilic molecules by connection of anelectrical circuit 26 to thecontacts electrical circuit 26 may have basically the same construction as a conventional circuit for performing stochastic sensing across a lipid bilayer formed in a conventional cell by the Montal & Mueller method. - An example design of the
electrical circuit 26 is shown inFIG. 12 . The primary function of theelectrical circuit 26 is to measure the electrical current signal developed between theelectrodes electrical circuit 26 needs to be sufficiently sensitive to detect and analyse currents which are typically very low. By way of example, an open membrane protein might typically pass current of 100 pA to 200 pA with a 1M salt solution. - In this implementation, the
electrode 24 in thechamber 7 is used as a reference electrode and theelectrode 21 in therecess 5 is used as a working electrode. Thus theelectrical circuit 26 provides theelectrode 24 with a bias voltage potential relative to theelectrode 21 which is itself at virtual ground potential and supplies the current signal to theelectrical circuit 26. - The
electrical circuit 26 has abias circuit 40 connected to theelectrode 24 in thechamber 7 and arranged to apply a bias voltage which effectively appears across the twoelectrodes - The
electrical circuit 26 also has anamplifier circuit 41 connected to theelectrode 21 in therecess 5 for amplifying the electrical current signal appearing across the twoelectrodes amplifier circuit 41 consists of a twoamplifier stages - The
input amplifier stage 42 connected to theelectrode 21 converts the current signal into a voltage signal. - The
input amplifier stage 42 may comprise transimpedance amplifier, such as an electrometer operational amplifier configured as an inverting amplifier with a high impedance feedback resistor, of for example 500 MΩ, to provides the gain necessary to amplify the current signal which typically has a magnitude of the order of tens to hundreds of picoamps. - Alternatively, the
input amplifier stage 42 may comprise a switched integrator amplifier. This is preferred for very small signals as the feedback element is a capacitor and virtually noiseless. In addition, a switched integrator amplifier has wider bandwidth capability. However, the integrator does have a dead time due to the necessity to reset the integrator before output saturation occurs. This dead time may be reduced to around a microsecond so is not of much consequence if the sampling rate required is much higher. A transimpedance amplifier is simpler if the bandwidth required is smaller. Generally, the switched integrator amplifier output is sampled at the end of each sampling period followed by a reset pulse. Additional techniques can be used to sample the start of integration eliminating small errors in the system. - The
second amplifier stage 43 amplifies and filters the voltage signal output by thefirst amplifier stage 42. Thesecond amplifier stage 43 provides sufficient gain to raise the signal to a sufficient level for processing in adata acquisition unit 44. For example with a 500 MΩ feedback resistance in thefirst amplifier stage 42, the input voltage to thesecond amplifier stage 43, given a typical current signal of the order of 100 pA, will be of the order of 50 mV, and in this case thesecond amplifier stage 43 must provide a gain of 50 to raise the 50 mV signal range to 2.5V. - The
electrical circuit 26 includes adata acquisition unit 44 which may be a microprocessor running an appropriate program or may include dedicated hardware. Thedata acquisition unit 44 may be a card to be plugged into acomputer 45 such as a desktop or laptop. In this case, thebias circuit 40 is simply formed by an inverting amplifier supplied with a signal from a digital-to-analog converter 46 which may be either a dedicated device or a part of thedata acquisition unit 44 and which provides a voltage output dependent on the code loaded into thedata acquisition unit 44 from software. Similarly, the signals from theamplifier circuit 41 are supplied to thedata acquisition card 40 through an analog-to-digital converter 47. - The various components of the
electrical circuit 26 may be formed by separate components or any of the components may be integrated into a common semiconductor chip. The components of theelectrical circuit 26 may be formed by components arranged on a printed circuit board. An example of this is shown inFIG. 13 wherein theapparatus 1 is bonded to a printedcircuit board 50 withaluminium wires 51 connecting from thecontacts tracks 52 on the printed circuit board. Achip 53 incorporating theelectrical circuit 26 is also bonded to the printedcircuit board 50. Alternatively theapparatus 1 and theelectrical circuit 26 may be mounted on separate printed circuit boards. - In the case that the
apparatus 1 containsplural recesses 5, each having arespective electrode 21, then theelectrical circuit 26 is modified essentially by replicating theamplifier circuit 41 and A/D converter 47 for eachelectrode 21 to allow acquisition of signals from eachrecess 5 in parallel. In the case that theinput amplifier stage 42 comprises switched integrators then those would require a digital control system to handle the sample-and-hold signal and reset integrator signals. The digital control system is most conveniently configured on a field-programmable-gate-array device (FPGA). In addition the FPGA can incorporate processor-like functions and logic required to interface with standard communication protocols i.e. USB and Ethernet. -
FIG. 14 shows a possible architecture of theelectrical circuit 26 and is arranged as follows. Therespective electrodes 21 of theapparatus 1 are connected to theelectrical circuit 26 by aninterconnection 55, for example thealuminium wires 51 and the printed circuit board in the arrangement ofFIG. 13 . In theelectrical circuit 26, theamplifier circuits 41 may be formed in one ormore amplifier chips 56 having plural channels. The signals fromdifferent electrodes 21 may be on separate channels or multiplexed together on the same channel. The outputs of the one ormore amplifier chips 56 are supplied via the A/D converter 47 to aprogrammable logic device 57 for receiving the signal on each channel. For example to handle signals from an apparatus having 1024 recesses, theprogrammable logic device 57 might operate at a speed of the order of 10 Mbits/s. Theprogrammable logic device 57 is connected via an interface 58, for example a USB interface, to acomputer 59 to supply the signals to thecomputer 59 for storage, display and further analysis. - During use the
apparatus 1 may be enclosed in a Faraday cage to reduce interference. - Various materials for the components of the
apparatus 1 will now be discussed. The materials for each component ofapparatus 1 are determined by the properties required to enable the component to function correctly during operation, but the cost and manufacturing throughput are also considered. All materials should be chosen to provide sufficient mechanical strength to allow robust handling, and surfaces compatible with bonding to the subsequent layers. - The material of the
substrate 3 is chosen to provide a rigid support for the remainder of theapparatus 1. The material is also chosen to provide a high resistance and low capacitance electrical insulation betweenadjacent electrodes 21 when there areplural recesses 5. Possible materials include without limitation: polyester (eg Mylar), or another polymer; or silicon, silicon nitride, or silicon oxide. For example, the substrate may comprise a silicon wafer with a thermally grown oxide surface layer. - The material of the further layer 4 (or in the general case layers) are chosen to provide a high resistance and low capacitance electrical insulation between the
electrodes plural recesses 5, between theelectrodes adjacent recesses 5. Also the surface of thefurther layer 4 should be chemically stable both to the pre-treatment coating applied before operation (as discussed below) and to theaqueous solution 10. Lastly, thefurther layer 4 should be mechanically robust in order to maintain its structural integrity and coverage of the firstconductive layer 20, and should be suitable for subsequent attachment of thecover 6. - The following is a list of possible materials for the
further layer 4, together with thicknesses which have been successfully employed experimentally, although these thicknesses are not limitative: photoresist (eg SU8 photoresist or Cyclotene) with a variety of thicknesses; polycarbonate, 6 μm thick film; PVC, 7 μm thick film; polyester, 50 μm thick film; adhesive backed polyester, 25 μm and 50 μm thick film; thermal laminating films, eg Magicard 15 μm thick and Murodigital 35 μm; or a screen-printed dielectric ink. - Advantageously, surfaces including (a) the outermost surface of the
body 2 around the recess and (b) the outer part of the internal surface of therecess 5 extending from the rim of therecess 5 are hydrophobic. This assists in the spreading of the pre-treatment coating and therefore also formation of a lipid bilayer. One particular way to achieve this is to modify these surfaces by a fluorine species. Such a fluorine species is any substance capable of modifying the surfaces to provide a fluorine-containing layer. The fluorine species is preferably one containing fluorine radicals. For example the modification may be achieved by treating thebody 2 with a fluorine plasma, for example a CF4 during manufacture. - The
conductive layers - The material of the
electrodes aqueous solution 10, enabling measurement of low currents, and should be stable to the pre-treatment coating andaqueous solution 10. The material of the remainder of theconductive layers 20 and 23 (usually but not necessarily the same as theelectrodes 21 and 24) also provides electrical conductance from the electrodes to thecontacts conductive layers 20 will also accept bonding of thefurther layers 4. Theconductive layers conductive layer 20 include without limitation: Silver/silver chloride electrode ink; silver with or without a surface layer, for example of silver chloride formed by chloridisation or of silver fluoride formed by fluoridisation; gold with or without redox couple in solution; platinum with or without redox couple in solution; ITO with and without redox couple in solution; gold electrochemically coated with conductive polymer electrolyte; or platinum electrochemically coated with conductive polymer electrolyte. Possible materials for the secondconductive layer 23 include without limitation: silver/silver chloride electrode ink; silver wire; or chloridised silver wire. - Some specific examples of include: the
substrate 3 being silicon and theconductive layer 20 being a metal conductor (diffusion or polysilicon wires are poor methods) buried in a silicon oxide insulating layer (e.g. using typical semiconductor fabrication technology); thesubstrate 3 being glass and theconductive layer 20 being metal conductors (e.g using typical LCD display technology); or thesubstrate 3 being a polymeric substrates and theconductive layer 20 being an ablated metal or printed conductor (e.g. using typical glucose biosensor technology). - The requirements for the material of the
cover 6 are to be easily attached to create a seal for thechamber 7, to be compatible with both the pre-treatment coating and theaqueous solution 10. The following are possible materials, together with thicknesses which have been successfully employed experimentally, although these thicknesses are not limitative: silicone rubber, 0.5, 1.0, 2.0 mm thick; polyester, 0.5 mm thick; or PMMA (acrylic) 0.5 mm to 2 mm thick. - Various methods of manufacturing the
apparatus 1 will now be discussed. In general terms, the layered construction of theapparatus 1 is simple and easy to form by a variety of methods. Three different fabrication technologies which have actually been applied are: lamination of polymer films; printed circuit board manufacture with high resolution solder mask formation and photolithography using silicon wafers or glass. - An example of a lamination process is as follows.
- The
substrate 3 is a 250 μm thick polyester sheet (Mylar), and the firstconductive layer 20 is deposited by either: screen printing silver/silver chloride electrode ink; adhesion of metal foil; or vapour deposition (sputtering or evaporation). Thefurther layer 4 is then laminated onto thesubstrate 3 by either: a pressure-sensitive adhesive; a thermally activated adhesive; or using the wet silver/silver chloride ink as the adhesive painted directly onto the dielectric before lamination (referred to as “painted electrodes”). The aperture in thefurther layer 4 that forms therecess 5 is created with 5-100 μm diameter either before or after lamination to thesubstrate 3 by either: electrical discharge (sparking); or laser drilling, for example by an excimer, solid state or CO2 laser. An apparatus created by lamination of polymer films sometimes requires an additional sparking step to activate the electrodes prior to use. The secondconductive layer 23 is formed on top of thefurther layer 4 by screen printing. Thecover 6 is laminated on top using pressure sensitive adhesive. - An example of a process employing photolithography using silicon wafers is as follows.
- The
substrate 3 is a silicon wafer with an oxide surface layer. The firstconductive layer 20 is formed by gold, silver, chloridised silver, platinum or ITO deposited onto thesubstrate 3. Photoresist (eg SU8) is then spin-coated over thesubstrate 3 to form thefurther layer 4. Therecess 5 is formed with 5-100 μm diameter by removal of the photoresist following UV exposure using a mask to define the shape of therecess 5. The secondconductive layer 23 is formed on top of thefurther layer 4, for example by screen printing. Thecover 6 is laminated on top using pressure sensitive adhesive. - The ability to use this type of process is significant because it allows the apparatus to be formed on silicon chips using standard silicon wafer processing technology and materials.
- The
electrodes - For stable and reliable operation, the
electrodes electrodes electrodes - Silver is a good choice for the material of
electrodes - Electroplating of silver may be achieved, for example, using a modified version of the method of Polk et al., “Ag/AgCl microelectrodes with improved stability for microfluidics”, Sensors and Actuators B 114 (2006) 239-247. A plating solution is prepared by addition of 0.41 g of silver nitrate to 20 ml of 1M ammonium hydroxide solution. This is rapidly shaken to avoid precipitation of the insoluble silver oxide, and to facilitate the formation of the diammine silver complex. The solution is always fresh to avoid fall in plating efficiency. The plating is performed using conventional equipment, connecting the
electrode 21 as the cathode and using a platinum electrode is used as the anode. For example in the case of plating on Pt electrodes, a potential of −0.58V is applied to the cathode, with the anode being held at ground potential, whereas in the case of plating on Au electrodes, the potential is held at −0.48V with respect to ground. A target charge of 5.1×103 C/m2 has been found empirically to result in a silver deposition of between 1 μm and 2 μm for a 100 μm diameter electrode, typically taking of the order of 60 s. - In performing such plating it is desirable to achieve uniform penetration of the aqueous plating solution to the bottom of the
recess 5. In the case that thelayer 4 is formed from a naturally hydrophobic material (eg SU8 photoresist) and in order to ensure uniform wetting of the recess, desirably the degree of hydrophilicity can be increased. Three methods to achieve this are as follows. A first method is application of a lipid to the surface of thelayer 4, so that the lipid acts as a surfactant, facilitating the entry of the plating solution. A second method is exposure of thelayer 4 to oxygen plasma which activates the material of the layer and produces hydrophilic functional groups. This produces a well defined hydrophilic and clean surface. A third method is to add ethanol to the plating solution. - Where the
electrode 21 is made of silver (or indeed other metals), the outer surface of the electrode is desirably converted to a halide, in order for theelectrode 21 to function efficiently as a provider of a stable reference potential. In common usage, the halide used is chloride, since the conversion of silver to silver chloride is relatively straightforward to achieve, for example by electrolysis in a solution of hydrochloric acid. Alternative chemical methods avoiding the use of a potentially corrosive acid which may affect the surface condition of thelayer 4 include a) sweeping voltammetry in 3M sodium chloride solution, and b) a chemical etching by immersion of theelectrode 21 in 50 mM ferric chloride solution. - An alternative halogen for the halidisation is fluorine. The choice of fluorine has the significant advantage that the silver fluoride layer can be formed in the same step as modification of surfaces (a) and (b) of the
body 2 to make them hydrophobic, as discussed above. For example this may be achieved during manufacture of theapparatus 1 by treatment of thebody 2 by a fluorine plasma for example a CF4 plasma. This is effective to modify the surfaces of thebody 2, particularly in the case that thelayer 4 is a photoresist such as SU8 to achieve a sufficient degree of hydrophobicity to support the formation of a stable lipid bilayer. At the same time exposure to the fluorine plasma converts the metal of theelectrode 21 into an outer layer of metal fluoride. - There will now be discussed some possible adaptations of the
electrode 21 in therecess 5 as alternatives to the use of a fluorine plasma as discussed above. - The
electrode 21 may be electrochemically modified to change the surface-type. This allows use of additional materials with good bulk properties but poor surface properties, such as gold. Possible electrochemical surface modifications include without limitation: silver electroplating; electrochemical chloridisation of silver; electropolymerisation of a polymer/polyelectrolyte. - By way of further example, one possible sequence of modification is shown in
FIG. 4 in which acoating 37 of silver is formed on theelectrode 21 formed of gold or platinum by electrochemical deposition. Electroplating may typically be performed in 0.2M AgNO2, 2M KI, 0.5 mM Na2S2O3 at −0.48V using a standard single liquid junction Ag/AgCl reference electrode and a platinum counter electrode. A typical thickness of thecoating 37 is estimated to be 750 nm with a deposition time of about 50 s and about 50 μC charge passed. Subsequently achloridised layer 38 is formed by chloridisation, typically at +150 mV in 0.1M HCl for 30 s. - Another possible surface modification is to apply a conductive polymer. The conductive polymer may be any polymer which is conductive. A suitable conductive polymer will have mobile charge carriers. Typically such a conductive polymer will have a backbone having delocalised electrons which are capable of acting as charge carriers, allowing the polymer to conduct. The conductive polymer may be doped to increase its conductivity, for example by a redox process or by electrochemical doping. Suitable conductive polymers include, without limitation: polypyrroles, polyacetylenes, polythiophenes, polyphenylenes, polyanilines, polyfluorenes, poly(3-alkylthiophene)s, polytetrathiafulvalenes, polynaphthalenes, poly(p-phenylene sulfide)s, polyindoles, polythionines, polyethylenedioxythiophenes, and poly(para-phenylene vinylene)s.
- One possible conductive polymer is a polypyrrole, which may be doped, for example with polystyrene sulfonate. This may be deposited, for example, on an electrode 21 of gold by electrooxidizing an aqueous solution of 0.1M pyrrole+90 mM polystyrene sulfonate in 0.1M KCl at +0.80V vs. Ag/AgCl reference electrode. The estimated thickness of polymer deposited is 1 μm at 30 μC, based on a assumption that 40 mC/cm2 of charge produces a film of thickness around 0.1 μm. The polymerization process can be represented as follows, where PE stands for polystyrene sulfonate:
- One advantage of using a conductive polymer deposited on an inert electrode, such as polypyrrole doped with polystyrene, electropolymerised onto gold or platinum, is to improve the electrode's performance as a stable electrode for conducting electrophysiological measurements. A further advantage is to increase the charge reservoir available to the electrode within the recess without increasing the volume of aqueous solution contained in the recess. These advantages are generally applicable when conducting electrophysiological measurements using an electrode in a recess, such as the
electrode 21 in theapparatus 1. - Other advantages of using a conductive polymer on the
electrode 21 in therecess 5 of theapparatus 1 include but are not limited to control of the hydrophilic nature of the electrode surface to aid wetting of the electrode surface by the aqueous buffer solution and similarly prevention of blocking of the electrode by the chemical pre-treatment prior to bilayer formation. -
FIGS. 34 a and 34 b are 3D and 2D surface profiles of an example electrode modified by electropolymerisation of polypyrrole, measured by profilometry. The thickness of electrochemically deposited polymer film in this example is about 2 μm.FIG. 35 shows the current recorded on an array of recesses modified by electropolymerisation of polypyrrole, showing stable lipid bilayers and single molecule detection of cyclodextrin from inserted protein pores. - In all embodiments, an alternative to the second
conductive layer 23 is to form an electrode in thechamber 7 simply by insertion through thecover 6 of a conductive member, such as a chloridised silver wire. - In order to characterise the
electrodes 21, visualisation ofrecesses 5 formed in abody 2 has been conducted using optical microscopy (OM), scanning electron microscopy (SEM), and laser profilometry (LP). -
FIG. 5 shows an SEM image of arecess 5 formed by drilling with a CO2 laser in anapparatus 1 formed by lamination of polymer layers, with subsequent application of electrical discharge to activate theelectrode 21. The image illustrates that the geometry of therecess 5 is poorly defined using this method of formation, with considerable surface damage therearound and variability in diameter, although it is hoped this may be improved through optimisation of the laser characteristics. -
FIG. 6 shows an OM image of arecess 5 formed using photolithography of afurther layer 4 of SU8 photoresist over anelectrode 21 of vapour deposited gold on asubstrate 3 of silicon. Similarly,FIGS. 7 a and 7 b are 3D and 2D LP profiles of a similarly manufacturedrecess 5.FIGS. 8 a and 8 b are 3D and 2D LP profiles of thesame recess 5 after electroplating to form acoating 38 of silver. These images show that photolithography provides a high degree of control of the geometry and dimensions of the recess. - Excimer laser methods also produce a controlled geometry similar to photolithography.
- There will now be described an example of a method of manufacture of the
apparatus 1, as shown inFIG. 33 . The rationale of this method is to provide high throughput manufacture. This is achieved by processing a wafer of silicon which forms thesubstrate 3 ofplural apparatuses 1 and which is subsequently diced. The wafer is prepared with an insulating layer, for example a thermally grown silicon-oxide. - First the wafer is prepared. In step S1, the wafer is cleaned. In step S2, the wafer is subjected to a HF dif to improve adhesion of metals and resist. Typical conditions are a 3 minute dip in 10:1 buffered oxide etch. In S3, the wafer is subjected to a bake as a dehydration step. Typical conditions are baking for 1 hour at 200° C. in an oven.
- Next, the wafer is metallised to provide the first
conductive layer 20 of eachapparatus 1. In step S4, photoresist is spun onto the wafer which is then subjected to UV light to form the desired pattern. In step S5, theconductive layers 20 are deposited, for example consisting of successive layers of Cr and Au. Typically ofrespective thicknesses 50 nm and 300 nm. In step S6 the resist is removed for example by soaking in acetone. - Next, the
layers 4 and recesses 5 are formed. In step S7, photoresist adhesion is improved by the application of an O2 plasma and dehydration bake for example in an oven. In step S8, the wafer has applied thereto photoresist which is then subjected to UV exposure to form thelayers 4 and recesses, for example SU8-10 with a thickness of 20 m. In step S9 an inspection and measurement of the recesses is performed. - Next, the
electrodes 21 are plated. In step S10, the surface is prepared for plating by performing an O2 plasma descum. In step S11, silver plating of the electrode is performed, as described above, for example to form a plating thickness of 1.5 μm. - In step S12, the wafer is diced to form the
bodies 2 ofseparate apparatuses 1. - Lastly, the
bodies 2 are treated by a CF4 plasma which modifies the surfaces of thebody 2 and theelectrode 21 as discussed above. A typical exposure is for 12 minutes at 70 W and 160 mTorr. - In practice with an
apparatus 1 manufactured using this method, the results of bilayer formation and pore current stability have been comparable to those achieved with bodies plated and chloridised by wet chemical means. - The method of using the
apparatus 1 to form alayer 11 of amphiphilic molecules will now be described. First the nature of the amphiphilic molecules that may be used will be considered. - The amphiphilic molecules are typically a lipid. In this case, the layer is a bilayer formed from two opposing monolayers of lipid. The two monolayers of lipids are arranged such that their hydrophobic tail groups face towards each other to form a hydrophobic interior. The hydrophilic head groups of the lipids face outwards towards the aqueous environment on each side of the bilayer. The bilayer may be present in a number of lipid phases including, but not limited to, the liquid disordered phase (fluid lamellar), liquid ordered phase, solid ordered phase (lamellar gel phase, interdigitated gel phase) and planar bilayer crystals (lamellar sub-gel phase, lamellar crystalline phase).
- Any lipids that form a lipid bilayer may be used. The lipids are chosen such that a lipid bilayer having the required properties, such as surface charge, ability to support membrane proteins, packing density or mechanical properties, is formed. The lipids can comprise one or more different lipids. For instance, the lipids can contain up to 100 lipids. The lipids preferably contain 1 to 10 lipids. The lipids may comprise naturally-occurring lipids and/or artificial lipids.
- The lipids typically comprise a head group, an interfacial moiety and two hydrophobic tail groups which may be the same or different. Suitable head groups include, but are not limited to, neutral head groups, such as diacylglycerides (DG) and ceramides (CM); zwitterionic head groups, such as phosphatidylcholine (PC), phosphatidylethanolamine (PE) and sphingomyelin (SM); negatively charged head groups, such as phosphatidylglycerol (PG); phosphatidylserine (PS), phosphatidylinositol (PI), phosphatic acid (PA) and cardiolipin (CA); and positively charged headgroups, such as trimethylammonium-Propane (TAP). Suitable interfacial moieties include, but are not limited to, naturally-occurring interfacial moieties, such as glycerol-based or ceramide-based moieties. Suitable hydrophobic tail groups include, but are not limited to, saturated hydrocarbon chains, such as lauric acid (n-Dodecanolic acid), myristic acid (n-Tetradecononic acid), palmitic acid (n-Hexadecanoic acid), stearic acid (n-Octadecanoic) and arachidic (n-Eicosanoic); unsaturated hydrocarbon chains, such as oleic acid (cis-9-Octadecanoic); and branched hydrocarbon chains, such as phytanoyl. The length of the chain and the position and number of the double bonds in the unsaturated hydrocarbon chains can vary. The length of the chains and the position and number of the branches, such as methyl groups, in the branched hydrocarbon chains can vary. The hydrophobic tail groups can be linked to the interfacial moiety as an ether or an ester.
- The lipids can also be chemically-modified. The head group or the tail group of the lipids may be chemically-modified. Suitable lipids whose head groups have been chemically-modified include, but are not limited to, PEG-modified lipids, such as 1,2-Diacyl-sn-Glycero-3-Phosphoethanolamine-N-[Methoxy(Polyethylene glycol)-2000]; functionionalised PEG Lipids, such as 1,2-Distearoyl-sn-Glycero-3 Phosphoethanolamine-N-[Biotinyl(Polyethylene Glycol)2000]; and lipids modified for conjugation, such as 1,2-Dioleoyl-sn-Glycero-3-Phosphoethanolamine-N-(succinyl) and 1,2-Dipalmitoyl-sn-Glycero-3-Phosphoethanolamine-N-(Biotinyl). Suitable lipids whose tail groups have been chemically-modified include, but are not limited to, polymerisable lipids, such as 1,2-bis(10,12-tricosadiynoyl)-sn-Glycero-3-Phosphocholine; fluorinated lipids, such as 1-Palmitoyl-2-(16-Fluoropalmitoyl)-sn-Glycero-3-Phosphocholine; deuterated lipids, such as 1,2-Dipalmitoyl-D62-sn-Glycero-3-Phosphocholine; and ether linked lipids, such as 1,2-Di-O-phytanyl-sn-Glycero-3-Phosphocholine.
- The lipids typically comprise one or more additives that will affect the properties of the lipid bilayer. Suitable additives include, but are not limited to, fatty acids, such as palmitic acid, myristic acid and oleic acid; fatty alcohols, such as palmitic alcohol, myristic alcohol and oleic alcohol; sterols, such as cholesterol, ergosterol, lanosterol, sitosterol and stigmasterol; lysophospholipids, such as 1-Acyl-2-Hydroxy-sn-Glycero-3-Phosphocholine; and ceramides. The lipid preferably comprises cholesterol and/or ergosterol when membrane proteins are to be inserted into the lipid bilayer.
- However, although lipids are commonly used to form bilayers, it is expected that in general the method is applicable to any amphiphilic molecules which may form a layer.
- As to the
aqueous solution 10, in general a wide range ofaqueous solutions 10 that are compatible with the formation of alayer 11 of amphiphilic molecules may be used. Theaqueous solution 10 is typically a physiologically acceptable solution. The physiologically acceptable solution is typically buffered to a pH of 3 to 11. The pH of theaqueous solution 10 will be dependent on the amphiphilic molecules used and the final application of thelayer 11. Suitable buffers include without limitation: phosphate buffered saline (PBS); N-2-Hydroxyethylpiperazine-N′-2-Ethanesulfonic Acid (HEPES) buffered saline; Piperazine-1,4-Bis-2-Ethanesulfonic Acid (PIPES) buffered saline; 3-(n-Morpholino)Propanesulfonic Acid (MOPS) buffered saline; and Tris(Hydroxymethyl)aminomethane (TRIS) buffered saline. By way of example, in one implementation, theaqueous solution 10 may be 10 mM PBS containing 1.0M sodium chloride (NaCl) and having a pH of 6.9. - The method of using the
apparatus 1 is as follows. - First, a
pre-treatment coating 30 is applied to thebody 2 across therecess 5, as shown inFIG. 9 . Thepre-treatment coating 30 is a hydrophobic fluid which modifies the surface of thebody 2 surrounding therecess 5 to increase its affinity to the amphiphilic molecules. - The
pre-treatment coating 30 is typically an organic substance, usually having long chain molecules, in an organic solvent. Suitable organic substances include without limitation: n-decane, hexadecane, isoecoisane, squalene, fluoroinated oils (suitable for use with fluorinated lipids), alkyl-silane (suitable for use with a glass membrane) and alkyl-thiols (suitable for use with a metallic membrane). Suitable solvents include but are not limited to: pentane, hexane, heptane, octane, decane, and toluene. The material might typically be 0.1 μl to 10 μl of 0.1% to 50% (v/v) hexadecane in pentane or another solvent, for example 2 μl of 1% (v/v) hexadecane in pentane or another solvent, in which case lipid, such as diphantytanoyl-sn-glycero-3-phosphocholine (DPhPC), might be included at a concentration of 0.6 mg/ml. - Some specific materials for the
pre-treatment coating 30 are set out in Table 1 by way of example and without limitation. -
TABLE 1 Pre-treatment formulation Volumes applied 0.3% hexadecane in pentane 2x 1 μl 1% hexadecane in pentane 2x2x 0.5 μl; 2x 0.5 μl; 1 μl; 2x 1 μl;2x 1 μl;2 μl; 2x 2 μl; 5μl 3% hexadecane in pentane 2x 1 μl; 2 μl 10% hexadecane in pentane 2x 1 μl; 2 μl; 5 μl 0.5% hexadecane + 0.6 mg/ml DPhPC lipid in 5 μl pentane 1.0% hexadecane + 0.6 mg/ml DPhPC lipid in 2x 2x 0.5 μl pentane 1.5% hexadecane + 0.6 mg/ml DPhPC lipid in 2 μl; 2x 1 μlpentane - The
pre-treatment coating 30 may be applied in any suitable manner, for example simply by capillary pipette. Thepre-treatment coating 30 may be applied before or after thecover 6 is attached to theapparatus 1. - The precise volume of material of the
pre-treatment coating 30 required depends on the size of therecess 5, the formulation of the material, and the amount and distribution of the when it dries around the aperture. In general increasing the amount (by volume and/or by concentration) improves the effectiveness, although excessive material can cover theelectrode 21 as discussed below. As the diameter of therecess 5 is decreased, the amount of material of thepre-treatment coating 30 required also varies. The distribution of thepre-treatment coating 30 can also affect effectiveness, this being dependent on the method of deposition, and the compatibility of the membrane surface chemistry. Although the relationship between thepre-treatment coating 30 and the ease and stability of layer formation is complex, it is straightforward to optimise the amount by routine trial and error. In another method thechamber 7 can be completely filled by pre-treatment in solvent followed by removal of the excess solvent and drying with a gas flow. - The
pre-treatment coating 30 is applied across therecess 5. As a result and as shown inFIG. 9 , thepre-treatment coating 30 covers the surface of thebody 2 around therecess 5. Thepre-treatment coating 30 also extends over the rim of therecess 5 and desirably covers at least the outermost portion of the side walls of therecess 5. This assists with formation of thelayer 11 of amphiphilic molecules across therecess 5. - However, the
pre-treatment coating 30 also has a natural tendency during application to cover theelectrode 21. This is undesirable as thepre-treatment coating 30 reduces the flow of current to theelectrode 21 and therefore reduces the sensitivity of measurement of electrical signals, in the worst case preventing any measurement at all. A number of different techniques may be employed to reduce or avoid this problem, and will be discussed after the description of forming thelayer 11 of amphiphilic molecules. - After application of the
pre-treatment coating 30, theaqueous solution 10 is flowed across thebody 2 to cover therecess 5 as shown inFIG. 3 . This step is performed with the amphiphilic molecules added to theaqueous solution 10. It has been demonstrated that, with an appropriatepre-treatment coating 30 this allows the formation of thelayer 11 of amphiphilic molecules across therecess 5. Formation is improved if a multi-pass technique is applied in whichaqueous solution 10 covers and uncovers therecess 5 at least once before covering therecess 5 for a final time. This is thought to be because at least some aqueous solution is left in therecess 5 which assists formation of thelayer 11 in a subsequent pass. Notwithstanding this, it should be noted that the formation of thelayer 11 is reliable and repeatable. This is despite the fact that the practical technique of flowingaqueous solution 10 across thebody 2 through thechamber 7 is very easy to perform. Formation of thelayer 11 may be observed by monitoring of the resultant electrical signals across theelectrodes layer 11 fails to form it is a simple matter to perform another pass of theaqueous solution 10. Such reliable formation of alayer 11 of amphiphilic molecules using a simple method and a relativelysimple apparatus 1 is a particular advantage of the present invention. - Furthermore, it has been demonstrated that the
layers 11 of amphiphilic molecules are of high quality, in particular being suitable for high sensitivity biosensor applications such as stochastic sensing and single channel recording. Thelayers 11 have high resistance providing highly resistive electrical seals, having an electrical resistance of 1 GΩ or more, typically at least 100 GΩ. which, for example, enable high-fidelity stochastic recordings from single protein pores. - This is achieved whilst trapping a volume of
aqueous solution 10 in therecess 5 between thelayer 11 and theelectrode 21. This maintains a significant supply of electrolyte. For example, the volume ofaqueous solution 10 is sufficient to allow stable continuous dc current measurement through membrane proteins inserted in the layer. - Experimental results demonstrating these advantages are set out later.
- There are various techniques for adding the amphiphilic molecules to the
aqueous solution 10, as follows. - A first technique is simply to add the amphiphilic molecules to the
aqueous solution 10 outside theapparatus 1 before introducing theaqueous solution 10 into thechamber 7. - A second technique which has particular advantage is, before introducing the
aqueous solution 10 into thechamber 7, to deposit the amphiphilic molecules on an internal surface of thechamber 7, or on an internal surface elsewhere in the flow path of theaqueous solution 10 into thechamber 7, for example in a fluidic inlet pipe connected to the inlet. The amphiphilic molecules can be deposited on any one or more of the internal surfaces of thechamber 7, including a surface of thefurther layer 4 or of thecover 6. Theaqueous solution 10 covers the internal surface during its introduction, whereby the amphiphilic molecules are added to theaqueous solution 10. In this manner, theaqueous solution 10 is used to collect the amphiphilic molecules from the internal surface. Theaqueous solution 10 may cover the amphiphilic molecules and therecess 5 in any order but preferably covers the amphiphilic molecules first. If the amphiphilic molecules are to be covered first, the amphiphilic molecules are deposited along the flow path between theinlet 8 and therecess 5. - Any method may be used to deposit the lipids on an internal surface of the
chamber 7. Suitable methods include, but are not limited to, evaporation or sublimation of a carrier solvent, spontaneous deposition of liposomes or vesicles from a solution and direct transfer of the dry lipid from another surface. Anapparatus 1 having lipids deposited on an internal surface may be fabricated using methods including, but not limited to, drop coating, various printing techniques, spin-coating, painting, dip coating and aerosol application. - The deposited amphiphilic molecules are preferably dried. In this case, the
aqueous solution 10 is used to rehydrate the amphiphilic molecules. This allows the amphiphilic molecules to be stably stored in theapparatus 1 before use. It also avoids the need for wet storage of amphiphilic molecules. Such dry storage of amphiphilic molecules increases shelf life of the apparatus. Even when dried to a solid state, the amphiphilic molecules will typically contain trace amounts of residual solvent. Dried lipids are preferably lipids that comprise less than 50 wt % solvent, such as less than 40 wt %, less than 30 wt %, less than 20 wt %, less than 15 wt %, less than 10 wt % or less than 5 wt % solvent. - In most practical uses, a membrane protein is inserted into the
layer 11 of amphiphilic molecules. There are several techniques for achieving this. - A first technique is simply for the
aqueous solution 10 to have a membrane protein added thereto, whereby the membrane protein is inserted spontaneously into thelayer 11 of amphiphilic molecules after a period of time. The membrane protein may be added to theaqueous solution 10 outside theapparatus 1 before introducing theaqueous solution 10 into thechamber 7. Alternatively the membrane protein may be added after formation of thelayer 11. - Another way of adding the membrane protein to the
aqueous solution 10 is to deposit it on an internal surface of thechamber 7 before introducing theaqueous solution 10 into thechamber 7. In this case, theaqueous solution 10 covers the internal surface during its introduction, whereby the membrane protein is added to theaqueous solution 10 and subsequently will spontaneously insert intolayer 11. The membrane proteins may be deposited on any one or more of the internal surfaces of thechamber 7, including a surface of thefurther layer 4 or of thecover 6. The membrane proteins can be deposited on the same or different internal surface as the amphiphilic molecules (if also deposited). The amphiphilic molecules and the membrane proteins may be mixed together. - Any method may be used to deposit the membrane proteins on an internal surface of the
chamber 7. Suitable methods include, but are not limited to, drop coating, various printing techniques, spin-coating, painting, dip coating and aerosol application. - The membrane proteins are preferably dried. In this case, the
aqueous solution 10 is used to rehydrate the membrane proteins. Even when dried to a solid state, the membrane proteins will typically contain trace amounts of residual solvent. Dried membrane proteins are preferably membrane proteins that comprise less than 20 wt % solvent, such as less than 15 wt % , less than 10 wt % or less than 5 wt % solvent. - A second technique is for the
aqueous solution 10 to have vesicles containing the membrane protein added thereto, whereby the membrane protein is inserted on fusion of the vesicles with thelayer 11 of amphiphilic molecules. - A third technique is to insert the membrane protein by carrying the membrane protein to the
layer 11 on a probe, for example an agar-tipped rod, using the techniques disclosed in WO-2006/100484. Use of a probe may assist in selectively inserting different membrane proteins indifferent layers 11, in the case that the apparatus has an array of recesses. However, this requires modification to theapparatus 1 to accommodate the probe. - Any membrane proteins that insert into a lipid bilayer may be deposited. The membrane proteins may be naturally-occurring proteins and/or artificial proteins. Suitable membrane proteins include, but are not limited to, β-barrel membrane proteins, such as toxins, porins and relatives and autotransporters; membrane channels, such as ion channels and aquaporins; bacterial rhodopsins; G-protein coupled receptors; and antibodies. Examples of non-constitutive toxins include hemolysin and leukocidin, such as Staphylococcal leukocidin. Examples of porins include anthrax protective antigen, maltoporin, OmpG, OmpA and OmpF. Examples of autotransporters include the NalP and Hia transporters. Examples of ion channels include the NMDA receptor, the potassium channel from Streptomyces lividans (KcsA), the bacterial mechanosensitive membrane channel of large conductance (MscL), the bacterial mechanosensitive membrane channel of small conductance (MscS) and gramicidin. Examples of G-protein coupled receptors include the metabotropic glutamate receptor. The membrane protein can also be the anthrax protective antigen.
- The membrane proteins preferably comprise α-hemolysin or a variant thereof. The α-hemolysin pore is formed of seven identical subunits (heptameric). The polynucleotide sequence that encodes one subunit of a-hemolysin is shown in SEQ ID NO: 1. The full-length amino acid sequence of one subunit of a-hemolysin is shown in SEQ ID NO: 2. The first 26 amino acids of SEQ ID NO: 2 correspond to the signal peptide. The amino acid sequence of one mature subunit of α-hemolysin without the signal peptide is shown in SEQ ID NO: 3. SEQ ID NO: 3 has a methionine residue at
position 1 instead of the 26 amino acid signal peptide that is present in SEQ ID NO: 2. - A variant is a heptameric pore in which one or more of the seven subunits has an amino acid sequence which varies from that of SEQ ID NO: 2 or 3 and which retains pore activity. 1, 2, 3, 4, 5, 6 or 7 of the subunits in a variant α-hemolysin may have an amino acid sequence that varies from that of SEQ ID NO: 2 or 3. The seven subunits within a variant pore are typically identical but may be different.
- The variant may be a naturally-occurring variant which is expressed by an organism, for instance by a Staphylococcus bacterium. Variants also include non-naturally occurring variants produced by recombinant technology. Over the entire length of the amino acid sequence of SEQ ID NO: 2 or 3, a variant will preferably be at least 50% homologous to that sequence based on amino acid identity. More preferably, the subunit polypeptide is at least 80%, at least 90%, at least 95%, at least 98%, at least 99% homologous based on amino acid identity to the amino acid sequence of SEQ ID NO: 2 or 3 over the entire sequence.
- Amino acid substitutions may be made to the amino acid sequence of SEQ ID NO: 2 or 3, for example a single amino acid substitution may be made or two or more substitutions may be made. Conservative substitutions may be made, for example, according to the following table. Amino acids in the same block in the second column and preferably in the same line in the third column may be substituted for each other:
-
NON-AROMATIC Non-polar G A P I L V Polar - uncharged C S T M N Q Polar - charged D E H K R AROMATIC H F W Y - Non-conservative substitutions may also be made at one or more positions within SEQ ID NO: 2 or 3, wherein the substituted residue is replaced with an amino acid of markedly different chemical characteristics and/or physical size. One example of a non-conservative substitution that may be made is the replacement of the lysine at position 34 in SEQ ID NO: 2 and
position 9 in SEQ ID NO: 3 with cysteine (i.e. K34C or K9C). Another example of a non-conservative substitution that may be made is the replacement of the asparagine residue atposition 43 of SEQ ID NO: 2 or position 18 of SEQ ID NO: 3 with cysteine (i.e. N43C or N17C). The inclusion of these cysteine residues in SEQ ID NO: 2 or 3 provides thiol attachment points at the relevant positions. Similar changes could be made at all other positions, and at multiple positions on the same subunit. - One or more amino acid residues of the amino acid sequence of SEQ ID NO: 2 or 3 may alternatively or additionally be deleted. Up to 50% of the residues residues may be deleted, either as a contiguous region or multiple smaller regions distributed throughout the length of the amino acid chain.
- Variants can include subunits made of fragments of SEQ ID NO: 2 or 3. Such fragments retain their ability to insert into the lipid bilayer. Fragments can be at least 100, such as 150, 200 or 250, amino acids in length. Such fragments may be used to produce chimeric pores. A fragment preferably comprises the β-barrel domain of SEQ ID NO: 2 or 3.
- Variants include chimeric proteins comprising fragments or portions of SEQ ID NO: 2 or 3. Chimeric proteins are formed from subunits each comprising fragments or portions of SEQ ID NO: 2 or 3. The β-barrel part of chimeric proteins are typically formed by the fragments or portions of SEQ ID NO: 2 or 3.
- One or more amino acid residues may alternatively or additionally be inserted into, or at one or other or both ends of, the amino acid sequence SEQ ID NO: 2 or 3. Insertion of one, two or more additional amino acids to the C terminal end of the peptide sequence is less likely to perturb the structure and/or function of the protein, and these additions could be substantial, but preferably peptide sequences of up to 10, 20, 50, 100 or 500 amino acids or more can be used. Additions at the N terminal end of the monomer could also be substantial, with one, two or more additional residues added, but more preferably 10, 20, 50, 500 or more residues being added. Additional sequences can also be added to the protein in the trans-membrane region, between amino acid residues 119 and 139 of SEQ ID NO: 3. More precisely, additional sequences can be added between residues 127 and 130 of SEQ ID NO: 3, following removal of residues 128 and 129. Additions can be made at the equivalent positions in SEQ ID NO: 2. A carrier protein may be fused to an amino acid sequence according to the invention.
- Standard methods in the art may be used to determine homology. For example the UWGCG Package provides the BESTFIT program which can be used to calculate homology, for example used on its default settings (Devereux et al (1984) Nucleic Acids Research 12, p 387-395). The PILEUP and BLAST algorithms can be used to calculate homology or line up sequences (such as identifying equivalent residues or corresponding sequences (typically on their default settings)), for example as described in Altschul S. F. (1993) J Mol Evol 36:290-300; Altschul, S. F et al (1990) J Mol Biol 215:403-10. Software for performing BLAST analyses is publicly available through the National Center for Biotechnology Information (https://www.ncbi.nlm.nih.gov/).
- The membrane proteins can be labelled with a revealing label. The revealing label can be any suitable label which allows the proteins to be detected. Suitable labels include, but are not limited to, fluorescent molecules, radioisotopes, e.g. 125I, 35S, enzymes, antibodies, polynucleotides and linkers such as biotin.
- The membrane proteins may be isolated from an organism, such as Staphylococcus aureus, or made synthetically or by recombinant means. For example, the protein may be synthesized by in vitro transcription translation. The amino acid sequence of the proteins may be modified to include non-naturally occurring amino acids or to increase the stability of the proteins. When the proteins are produced by synthetic means, such amino acids may be introduced during production. The proteins may also be modified following either synthetic or recombinant production.
- The proteins may also be produced using D-amino acids. In such cases the amino acids will be linked in reverse sequence in the C to N orientation. This is conventional in the art for producing such proteins.
- A number of side chain modifications are known in the art and may be made to the side chains of the membrane proteins. Such modifications include, for example, modifications of amino acids by reductive alkylation by reaction with an aldehyde followed by reduction with NaBH4, amidination with methylacetimidate or acylation with acetic anhydride.
- Recombinant membrane proteins can be produced using standard methods known in the art. Nucleic acid sequences encoding a protein can be isolated and replicated using standard methods in the art. Nucleic acid sequences encoding a protein can be expressed in a bacterial host cell using standard techniques in the art. The protein can be introduced into a cell by in situ expression of the polypeptide from a recombinant expression vector. The expression vector optionally carries an inducible promoter to control the expression of the polypeptide.
- Thus the
apparatus 1 can be used for a wide range of applications. Typically a membrane protein is inserted in thelayer 11. An electrical signal, typically a current signal, developed between theelectrode 21 in therecess 5 and thefurther electrode 24 in thechamber 7 is monitored, using theelectrical circuit 26. Often a voltage is also applied between theelectrodes layer 11 and any membrane protein inserted therein. - Some non-limitative examples of uses will now described. One use is in vitro investigation of membrane proteins by single-channel recording. An important commercial use is as a biosensor to detect the presence of a range of substances. The
apparatus 1 may be used to detect an analyte molecule that binds with an inserted membrane protein, or another stimulus, using stochastic sensing by detecting a change in the current flow indicating the presence of the analyte molecule or other stimulus. Similarly, theapparatus 1 may be used to detect the presence or absence of membrane pores or channels in a sample, by detecting a change in the current flow as the pore or channel inserts. The lipid bilayer may be used for a range of other purposes, such as studying the properties of molecules known to be present (e.g. DNA sequencing or drug screening), or separating components for a reaction. - Some techniques to reduce or avoid the problem of the
pre-treatment coating 30 covering theelectrode 21 will now be discussed. - A first technique is, after application of the
pre-treatment coating 30 to apply a voltage across theelectrode 21 in therecess 5 and thefurther electrode 24 in thechamber 7 sufficient to reduce the amount of excess hydrophobic fluid covering theelectrode 21 in therecess 5. This is produces a similar effect to electro-wetting. - This technique is illustrated in
FIGS. 10 a to 10 e. First, as shown inFIG. 10 a, thepre-treatment coating 30 is applied as shown inFIG. 10 a where thepre-treatment coating 30 covers theelectrode 21. Next, as shown inFIG. 10 b,aqueous solution 10 is flowed across thebody 2 to cover therecess 5 so thataqueous solution 10 flows into therecess 5. Next, a voltage is applied which removes thepre-treatment coating 30 covering theelectrode 21, as shown inFIG. 10 c. This voltage will rupture any layer of amphiphilic molecules formed across therecess 5. Therefore, next, as shown inFIG. 10 d, theaqueous solution 10 is flowed out of thechamber 7 to uncover therecess 5. Typically an amount ofaqueous solution 10 will remain in therecess 5. Lastly, as shown inFIG. 10 e,aqueous solution 10, having amphiphilic molecules added thereto, is flowed across thebody 2 to re-cover therecess 5 so that thelayer 11 of the amphiphilic molecules forms. - This is most simply performed by flowing the same
aqueous solution 10 in and out of thechamber 7. However, in principle, theaqueous solution 10 flowed into thechamber 7 to re-covering the recess 5 (inFIG. 10 e) could be different from theaqueous solution 10 flowed into thechamber 7 to first cover the recess 5 (inFIG. 10 b) before applying the voltage. Similarly, there could be no amphiphilic molecules added to theaqueous solution 10 flowed into thechamber 7 to first cover the recess 5 (inFIG. 10 b) before applying the voltage. - A second technique is to make an inner part of the internal surface of the
recess 5 hydrophilic. This may be achieved by making thebody 2 with two (or in general more)further layers FIG. 11 , of which the innermostfurther layer 4 a (or layers) formed of a hydrophilic material, for example SiO2. Typically but without limitation, the innermostfurther layer 4 a might have a thickness of 2 μm. - The outermost
further layer 4 b (or layers) is formed of a hydrophobic material and as a result both of (a) the outermost surface of thebody 2 around the recess and (b) the outer part of the internal surface of therecess 5 extending from the rim of therecess 5 is hydrophobic. This assists in the spreading of the pre-treatment coating. Indeed this property of these surfaces of thebody 2 is desirable even if there is not an innerfurther layer 4 a formed of a hydrophilic material. Typically but without limitation, outermostfurther layer 4 b might have a thickness of 1 μm, 3 μm, 5 μm, 10 μm, 20 μm or 30 μm. - A third technique is to provide a hydrophillic surface on the
electrode 21 which repels the appliedpre-treatment coating 30, whilst allowing ionic conduction from theaqueous solution 10 to theelectrode 2. This may be achieved by depositing a protective material on theelectrode 21. A range of protective materials may be used. One possibility is a conductive polymer, for example polypyrrole/polystyrene sulfonate as discussed above. Another possibility is a covalently attached hydrophilic species, such as thiol-PEG. - The
apparatus 1 described above has been made and used experimentally to demonstrate formation of alayer 11, in particular being a lipid bilayer, and insertion of a membrane protein, in particular α-hemolysin. The following procedure was followed after manufacture of the apparatus 1: - 1) apply
pre-treatment coating 30 tobody 2; - 2) introduce
aqueous solution 10 intochamber 7 to coverrecess 5; - 3) electro-wet the
electrode 21; - 4) remove
aqueous solution 10 toun-cover recess 5 and re introduceaqueous solution 10 intochamber 7 to coverrecess 5 and form thelayer 11; - 5) add α-hemolysin free into
aqueous solution 10 and monitor insertion intolayer 11. - In step 1), the
pre-treatment coating 30 was hexadecane dissolved in pentane. The quantity and volume of thepre-treatment coating 30 was varied for each test to obtain the optimum conditions for formation of thelayer 11. Insufficientpre-treatment coating 30 prevented formation of thelayer 11 while excesspre-treatment coating 30 caused blocking of the recesses. However routine variation of the amount allowed optimisation. - The amphiphilic molecules were a lipid, in particular 1,2-diphytanoyl-sn-glycero-3-phosphocholine. The lipid was dissolved in pentane and then dried onto the surface of the
cover 6 defining an internal surface of thechamber 7 before attaching thecover 6 on top of thebody 2. In step 2), theaqueous solution 10 collected the lipid. - Step 3) was performed by application of a large potential to across the
electrodes pre-treatment coating 30 from theelectrode 21. Although not required in every case, when performed this stage helped to condition therecess 5 for formation of thelayer 11 and assisted subsequent measurement of electrical signals. - By monitoring of the electrical signals developed across the
electrodes layer 11 and insertion of the membrane protein was observed. - The procedure was successfully performed for an
apparatus 1 of the type described above formed by lamination onto apolymer substrate 3. Formation of thelayer 11 and insertion of the membrane protein was observed using all the fabrication variables described above, albeit with varying degrees of repeatability and signal quality. - An example will now be described for a
typical apparatus 1, in which the firstconductive layer 20 was formed by a silver foil strips (25 μm thick, from Goodfellow) thermally laminated onto thesubstrate 3 using a 15 μm thick laminating film (Magicard) to form thefurther layer 4. Acircular recess 5 ofdiameter 100 μm was createdfurther layer 4 using an excimer laser, exposing acircular silver electrode 21 ofdiameter 100 μm. The exposed silver was chloridised electrochemically as described previously. The secondconductive layer 23 was a screen printing silver/silver chloride ink printed on the top side of thebody 2. - The
pre-treatment coating 30, comprising 0.5 μl of 1% heaxadecane +0.6 mg/ml DPhPC in pentane, was then applied to thebody 2 and dried at room temperature. - The
cover 6 comprised a 1 mm thick silicon rubber body with a 250 μm thick Mylar lid. Lipid (4 μl of 10 mg/ml DPhPC in pentane) was applied to the inside of thecover 6 and allowed to dry at room temperature before attachment to thebody 2 with self-adhesive. - A typical successful test proceeded as follows.
- The
dry contacts electrical circuit 26 enclosed in a Faraday cage and a 20mV 50 Hz triangular potential waveform applied.FIG. 15 shows the applied waveform and the resultant current signal which is indicative of the expected capacitive response. - Addition of the
aqueous solution 10 creates an “open circuit” connection between the electrodes, such that the current response to the applied potential waveform is large, typically saturating the current amplifier. A typical trace is shown inFIG. 16 , involving a current response greater than 20,000 pA to the 20 mV potential. This corresponds to a resistance of less than 1 MΩ, which is sufficiently small for use in conjunction with bilayer formation and pore current measurement. - In the event that the
electrode 21 does not initially form a proper electrical connection with theaqueous solution 10, application of a −1V DC potential can be used to increase in the available active electrode area. This is illustrated inFIG. 17 , in which the electrode begins partially active and is then fully activated after around 4 s of the applied potential. - Following open-circuit connection between the
aqueous solution 10 and theelectrode 21, theaqueous solution 10 is removed from thechamber 7 and reintroduced. On re-introduction, alayer 11 of the lipid collected from the internal surface of thechamber 7 is formed across therecess 5. The formation is observed by an increase in the capacitive squarewave current response to just under 500 pA, for example as shown inFIG. 18 . This value is consistent with the capacitance expected for a circular lipid bilayer of diameter oforder 100 μm and varies predictably for different geometries. - Subsequent addition of α-hemolysin to the
aqueous solution 10 creates a current response typical of pore insertion under an applied potential of 100 mV. For exampleFIG. 19 is a typical example with cyclodextrin present in theaqueous solution 10 and shows an expected current response with binding events confirming that the current is through the pores. - Although the example above shows data for the thermally
laminated apparatus 1, the other systems investigated also produced successful formation of thelayer 11 and pore insertion. For example, this was also successfully demonstrated for anapparatus 1 formed by lamination using pressure-sensitive adhesive bonding of thefurther layer 4. However, the adhesive layer was found to complicate formation of therecess 5 both in terms of the resulting aspect ratio and spreading of the adhesive across theelectrode 21. This problem was overcome by electrical sparking to “activate” theelectrode 21. - The impact of the quality of the
recess 5 is evident by comparing results from recesses formed by a CO2 laser and an excimer laser, as shown inFIGS. 20 and 21 , respectively. In both cases formation of thelayer 11 and pore insertion is successful and evident in the response, but more reproducible apertures were produced using the excimer laser.Recesses 5 formed by the CO2 laser tended to form relativelyleaky layers 11 with more noisy pore signals and were also susceptible to blocking.Recesses 5 formed by the excimer laser produced well sealedlayers 11 with good pore signals. - Formation of the
layer 11 and pore insertion was similarly observed with anapparatus 1 formed as described above using high definition printed circuit board manufacture. In this case, to formapparatus 1, the firstconductive layer 20 was formed by etching the copper foil on an FR4 substrate typically used in printed circuit board manufacture. The board was then screen printed with a Ronascreen SPSR™ photoimageable solder mask to a depth of 25 μm and exposed to UV light on an Orbotech Paragon 9000 laser direct imaging machine and developed with KaCO3 solution to create 100 μm circular apertures over theelectrodes 21. - Formation of the
layer 11 and pore insertion was similarly observed with anapparatus 1 formed as described above using photolithography. In this case, to form theapparatus 1, the firstconductive layer 20 was formed by gold vapour deposited using clean-room facilities onto thesubstrate 3 and afurther layer 4 of SU8 photoresist of thickness 12.5 μm was spin-coated on top.Recesses 5 were formed by curing of the photoresist by UV exposure with a mask and subsequent removal of the uncured photoresist. Therecesses 5 had a diameter of 100 μm, exposing anelectrode 21 ofdiameter 100 μm. After baking to set the photoresist, the wafer was diced to form separate substrates each with asingle recess 5. Theelectrodes 21 were electroplated with silver and then chloridised electrochemically as described previously. Thesecond electrode 24 was screen printed silver/silver chloride ink printed on the top side of thebody 2. - The
pre-treatment coating 30, comprising 0.5 μl of 0.75% hexadecane in pentane, was then applied to thebody 2 and dried at room temperature. - The
cover 6 comprised a 1 mm thick silicon rubber body with a 250 μm thick Mylar lid. Lipid (40 of 10 mg/ml DPhPC in pentane) was applied to the inside of thecover 6 and allowed to dry at room temperature before attachment to thebody 2 with self-adhesive. - Testing was performed as described above and successful formation of the
layer 11 and pore insertion was observed. For example,FIG. 22 shows a typical current trace showing cyclodextrin binding events with wild-type α-hemolysin pores. - These results generally show the ease with which the method of formation of the
layer 11 may be performed. In particular formation of thelayer 11 is achieved with a wide range of materials of theapparatus 1, dimensions (width and depth) of therecess 5, and methods of manufacture. Some variation in success rate is evident but in general this can be optimised by routine testing ofdifferent apparatuses 1. In particular the formation of thelayer 11 is not overly dependent on the width of therecess 5. Formation has been demonstrated over widths from 5 μm to 100 μm and in view of the ease of formation it is expected that formation is possible at higher widths up to 200 μm, 500 μm or higher. Also in view of this ease of formation of thelayer 11, it is expected that variations of the shape of therecess 5 could also be accommodated. - There will now be discussed modifications to the
apparatus 1 to includeplural recesses 5, commonly referred to as an array ofrecesses 5. The ability to easily form an array oflayers 11 across an array ofrecesses 5 in asingle apparatus 1 is a particular advantage of the present invention. By contrast to traditional methods of formation of lipid bilayers, theapparatus 1 has asingle chamber 7, but creates thelayer 11 in situ during the test and captures a reservoir of electrolyte in therecess 5 under thelayer 11 which allows continuous stable measurement of current passing through protein pores inserted in thelayer 11. Further thelayer 11 formed is of high quality and is localised to the area of therecess 5, ideal for high-fidelity current measurements using membrane protein pores. These advantages are magnified in anapparatus 1 which forms an array oflayers 11 because this allows measurements to be taken across all thelayers 11 in parallel, either combining the current signals to increase sensitivity or monitoring the current signals separately to perform independent measurements across eachlayer 11. - Apparatuses having an array of
recesses 5 have been tested and demonstrated successful formation of an array oflayers 11, showing the possibility of creating a miniaturised array of close packed individually addressable layers recording current signals in parallel from a test sample. - Essentially an
apparatus 1 having an array ofrecesses 5 can be formed simply using the manufacturing techniques described above but instead formingplural recesses 5. In this case, the firstconductive layer 20 is divided to form aseparate electrode 21,contact 22 and intermediateconductive track 27 in respect of eachrecess 5. Theapparatus 1 has asingle chamber 7 with asingle electrode 24 common to all therecesses 5. -
FIGS. 23 to 25 show first to third designs in which theapparatus 1 is modified by providing, respectively, four, nine and 128recesses 5 in thefurther layer 4. In each of the first to third designs, the firstconductive layer 20 is divided, as shown, respectively, inFIGS. 26 to 28 being plan views of thesubstrate 3. The firstconductive layer 20 provides, in respect of each recess 5: anelectrode 21 underneath therecess 5; acontact 22 exposed for connection of theexternal circuit 26 and atrack 27 between theelectrode 21 and thecontact 22. Thus eachelectrode 21, and its associatedtrack 27 andcontact 22, is electrically insulated from each other allowing separate measurement of current signals from eachrecess 5. - Manufacture of the
apparatus 1 may be performed using the techniques described above using lamination of polymer films or photolithography using silicon wafers. -
Apparatuses 1 havingplural recesses 5 have been made and used experimentally to demonstrate formation of alayer 11, in particular being a lipid bilayer, and insertion of a membrane protein, in particular α-hemolysin. The experimental procedure was as described above for anapparatus 1 having asingle recess 5, except that formation of thelayer 5 and membrane protein insertion was observed atplural recesses 5. Some examples are as follows. - An apparatus of the first design having four
recesses 5 was manufactured by the technique described above of lamination onto apolymer substrate 3. The firstconductive layer 20 was silver vapour deposited on apolyester sheet substrate 3. Thefurther layer 4 was a 15 μm thick laminating film thermally laminated on top. The fourrecesses 5 of 100 μm diameter were formed at a pitch of 300 μm by an excimer laser. - For recording of from each
recess 5 simultaneously in parallel, multiple Axon current amplifier devices were operated in parallel with a single silver/silver chloride electrode 24 in thechamber 7 as the ground electrode common to all channels. Formation oflayers 11 and insertion of membrane proteins atplural recesses 5 was successfully recorded in parallel. Often this occurred at eachrecess 5 although sometimes alayer 11 failed to form at one ormore recesses 5. For example typical current traces are shown inFIG. 29 demonstrating simultaneous formation of fourlayers 11, each having one or two α-hemolysin pores inserted, with cyclodextrin binding events. Notably there is no cross-talk between the signals. This confirms that thelayers 11 are operating independently and can produce meaningful measurements in parallel while being individually addressed and using a commonsecond electrode 24. - An apparatus of the second design having nine
recesses 5 was manufactured by the technique described above of photolithography usingsilicon wafer substrates 2. Thefurther layer 4 was 5 μm thick SU8 photoresist. The ninecircular recesses 5 were formed at a pitch of 300 μm by photolithography. In this case, therecesses 9 had different diameters, in particular of 5 μm, 10 μm, 15 μm, 20 μm, 20 μm, 30 μm, 40 μm, 50 μm, and 100 μm. Thesubstrate 3 was bonded to a printed circuit board with separate tracks connected to eachcontact contacts - In order to control the applied potential and record the current response in parallel, a multichannel
electrical circuit 26 was created with corresponding software. Testing was computer automated using a syringe pump to provide fluidics control of the repeated application and removal of theaqueous solution 10. - Formation of
layers 11 and insertion of membrane proteins atplural recesses 5 was successfully recorded in parallel. Often this occurred at eachrecess 5 although sometimes alayer 11 failed to form at one ormore recesses 5. For example, typical current traces forrecesses 5 constructed with gold electrodes and operating without a redox couple in solution are shown inFIG. 30 demonstrating simultaneous formation of eightlayers 11, each having one or two α-hemolysin pores inserted, with cyclodextrin binding events. Again there is no cross-talk and this confirms that thelayers 11 are operating independently and can produce meaningful measurements in parallel. - Furthermore the
apparatus 1 demonstrates successful formation of alayer 11 across therecess 5 of each diameter in the range of 5 μm to 100 μm. Accordingly theapparatus 1 was used to investigate the role of the diameter of therecess 5 and the quantity of pre-treatment coating applied, by experimentally testing the percentage success rate of forming alayer 5 with three different concentrations ofpre-treatment coating 30, namely 0.5%, 1.0%, and 2.0% hexadecane in pentane. The results showed that in the case of too littlepretreatment coating 30, it was not possible to form thelayer 11 across the range of diameters ofrecess 5. Furthermore in the case of toomuch pretreatment coating 30, it was not possible to wet theelectrode 21 and formation of thelayer 11 could not be observed. In this particular configuration, the yield of formation oflayers 11 was greater than 60% for the range of diameters 15 μm to 100 μm. Factors affecting layer formation, some of which were investigated in this experiment include, but are not limited to,pretreatment coating 30, diameter ofrecess 5, depth ofrecess 5, aspect ratio ofrecess 5, surface properties of therecess 5, surface properties of the surfaces around the recess, fluid flow within thechamber 7, the amphiphilic molecules used in the layer formation and the physical and electrical properties of theelectrode 21 within therecess 5. Subsequent experiments have demonstrated yield of formation oflayers 11, verified by stochastic binding signals of inserted membrane channels, greater than 70% using the 128 recesses, each 100 μm in diameter, of the device ofFIG. 28 . - In the
apparatus 1 described above, theconductive tracks 27 from theelectrode 21 to thecontact 22 is formed on a surface of thesubstrate 3 under the further layer. This may be referred to as a planar escape route for theconductive track 27. As previously described the separateconductive tracks 27 allow eachelectrode 21 to be connected individually to a dedicated low-noise high-input impedance picoammeter in thecircuit 26 whilst minimising the signal deterioration due to noise and bandwidth reduction. Such planarconductive tracks 27 are ideal for anapparatus 1 having a small number ofrecesses 5 and a thick layer between thetracks 27 and theaqueous solution 10. - However, for uses where high sensitivity is required, the electrical connection between the
electrodes 21 and the amplifier circuit desirably has low parasitic capacitance and low leakage to the surroundings. Parasitic capacitance causes noise and hence signal deterioration and bandwidth reduction. Leakage also increases noise, as well as introducing an offset current. In theapparatus 1, theconductive tracks 27 experience some degree of parasitic capacitance and leakage, both betweentracks 27 and between track andaqueous solution 10. As the number of recesses in the array increases, the number of electrical connections to escape increases and with a planar escape route, a practical limit is reached where the density of theconductive tracks 27 creates too much parasitic capacitance and/or leakage between tracks. Furthermore as the thickness of thelayer 4 decreases the capacitance and/or leakage between thetracks 27 and theaqueous solution 10 increases. - By way of example, typical figures may be obtained by modelling the lipid bilayer as a capacitive element with a typical value for the capacitance per unit area of 0.8 μF/cm2. The parasitic capacitance between
track 27 andaqueous solution 10 can be crudely modelled as a capacitative element with the area oftrack 27 exposed, through the layer, to the aqueous solution. Typical values for thetrack 27 may be 50 μm wide with 2 mm exposed and a relative permittivity (dielectric constant) of the layer around 3. For a 100 μm diameter bilayer and 20 μm deep recess the capacitance is 63 pF with a track-solution parasitic capacitance of 0.13 pF. However scaling to smaller bilayers of 5 μm diameter and 1 μm deep the capacitance is 0.16 pF with parasitic capacitance 0.53 pF. For smaller bilayers and thinner layers the parasitic capacitance dominates. - To reduce this problem, a modification shown in
FIG. 31 is to replace theconductive track 27 by aconductive path 28 which extends through thebody 2 to acontact 29 on the opposite side of thebody 2 from theelectrode 21. In particular, theconductive path 28 extends through thesubstrate 3. As thissubstrate 3 provides a thicker dielectric between theconductive paths 28 than is possible between the planarconductive paths 27, a much lower parasitic capacitance is achieved. Also, the leakage is low due to the thickness and dielectric properties of thesubstrate 3. Consequently, the use of theconductive paths 28 effectively increases the number ofrecesses 5 which may be accomodated in thebody 2 before the practical limits imposed by parasitic capacitance and/or leakage are met. This form of interconnect can be attached to a low-capacitance multi-layer substrate 61, which allows a far greater number of electrical escape routes by virtue of the number of layers and the low dielectric constant of the material. In addition the use of solder bump technology (also known as “flip chip” technology) and a suitable connector allows theapparatus 1 shown inFIG. 31 , excluding thesubstrate 61, to be made as low cost disposable part. - The
conductive path 28 may be formed using known through-wafer interconnection technology. Types of through-wafer interconnects which may be applied to form the conductive path include without limitation: - on
substrates 3 of silicon, through-wafer interconnects formed by producing a via through the silicon wafer, isolating the internal surface of via and filling the via with a conducting material, or alternatively theconductive path 28 is formed by producing a semiconductor PN junction in the form of a cylindrical via through the silicon substrate; - on
substrates 3 of glass, through-wafer interconnects formed by methods including laser drilling, wet etching and filling vias with metal or doped semiconductor material; and - on
substrates 3 made of polymers, through-wafer interconnects formed by methods including laser drilling, laser ablation, screen printed conductors and known printed circuit board techniques. - As the opposite side of the
body 2 from theelectrode 21 is dry, an electrical point contact array can be used to make connections to theelectrical circuit 26. By way of example,FIG. 31 illustrates the use of solder bump connections. In particular, deposited on eachcontact 29 are respective solder bumps 60 on which acircuit element 61 is mounted so that the solder bumps 60 make electrical contact with atrack 62 on thecircuit element 61. - The
circuit element 61 may be a printed circuit board for example as shown inFIG. 13 . - Alternatively, the
circuit element 61 could be an integrated circuit chip or a laminate, for example a low temperature cured ceramic package. Such an integrated circuit chip or laminate may be used as a method of spreading out connections, connecting to a further solder bump array on the opposite side of the integrated circuit chip or laminate with a greater pitch. An example of this is shown inFIG. 32 in which thecircuit element 61 is an integrated circuit chip or a laminate providing connections from the solder bumps 60 deposited on thebody 2 to further solder bumps 63 arrayed at a greater pitch and used to connect to afurther circuit element 64, for example a printed circuit board. Thecircuit element 61 being an integrated circuit chip or laminate may also be used to escape connections sideways in a multi-layer format. - In the case of a
substrate 3 of semiconductor material such as silicon, two types of through-wafer interconnect which may be applied to make theconductive path 28 are Metal-Insulator-Semiconductor (MIS), and a PN junction type. In MIS, a hole is drilled through the silicon chip by Deep Reactive Ion Etching (DRIE) process and this hole is coated with insulator and then filled with metal to form theconductive path 28. The PN junction type of through-wafer interconnect is a semiconductor junction formed into a cylindrical via through a silicon chip. Each type of through-wafer interconnection is formed on silicon wafers that have been thinned down to less than 0.3 mm to save DRIE processing time in making the holes. The important feature of PN junction type through-wafer interconnects is the low capacitance provided by having a large depletion region compared to the MIS type of interconnect. This is partially helped by increasing the reverse-bias of the junction.
Claims (33)
1. A method of forming a layer separating two volumes of aqueous solution, the method comprising:
(a) providing an apparatus comprising elements defining a chamber, the elements including a body of non-conductive material having formed therein at least one recess opening into the chamber, the recess containing an electrode;
(b) applying a pre-treatment coating of a hydrophobic fluid to the body across the recess;
(c) flowing aqueous solution, having amphiphilic molecules added thereto, across the body to cover the recess so that aqueous solution is introduced into the recess from the chamber and a layer of the amphiphilic molecules forms across the recess separating a volume of aqueous solution introduced into the recess from the remaining volume of aqueous solution.
2. A method according to claim 1 , wherein step (c) comprises:
(c1) flowing aqueous solution across the body to cover the recess so that aqueous solution flows into the recess;
(c2) flowing the aqueous solution to uncover the recess, leaving some aqueous solution in the recess; and
(c3) flowing aqueous solution that is optionally the same aqueous solution as in step (c2), having amphiphilic molecules added thereto, across the body and to re-cover the recess so that a layer of the amphiphilic molecules forms across the recess separating a volume of aqueous solution inside the recess from the remaining volume of aqueous solution.
3. A method according to claim 2 , wherein
the apparatus is provided with a further electrode in the chamber outside said recess, in step (c1), the aqueous solution is flowed also to contact the further electrode, and step (c) further comprises, between steps (c1) and (c2):
(c4) applying a voltage across said electrode contained in the recess and said further electrode sufficient to reduce the amount of excess hydrophobic fluid covering said electrode contained in the recess.
4. (canceled)
5. A method according to claim 1 , wherein surfaces including one or both of (a) the outermost surface of the body around the recess, and (b) at least an outer part of the internal surface of the recess extending from the rim of the recess, are hydrophobic.
6. A method according to claim 5 , wherein the body comprises an outermost layer formed of a hydrophobic material, the recess extending through the outermost layer and said outer part of the internal surface of the recess being a surface of the outermost layer.
7. A method according to claim 5 , wherein an inner part of the internal surface of the recess inside the outer part is hydrophilic.
8.-11. (canceled)
12. A method according to claim 1 , wherein the body comprises a substrate and at least one further layer attached to the substrate, the recess extending through the at least one further layer.
13. A method according to any claim 1 , wherein the electrode has provided thereon a hydrophillic surface which repels the hydrophobic fluid applied in step (c) whilst allowing ionic conduction from the aqueous solution to the electrode.
14.-18. (canceled)
19. A method according to claim 1 , wherein the internal surface of the 15 recess has no openings capable of fluid communication.
20.-23. (canceled)
24. A method according to claim 1 , further comprising, before step (c), depositing the amphiphilic molecules on an internal surface of the chamber or on an internal surface 30 in the flow path of the aqueous solution into the chamber, the aqueous solution covering the internal surface during step (c) whereby the amphiphilic molecules are added to the aqueous solution.
25.-27. (canceled)
28. A method according to claim 1 , wherein the at least one recess comprises plural recesses and the method comprises inserting different membrane protein into the layers of amphiphilic molecules formed in different recesses.
29. A method according to claim 1 , further comprising inserting a membrane protein into the layer of amphiphilic molecules and wherein the apparatus is provided with a further electrode in the chamber outside the recess, and the method further comprises applying a potential across the electrode in the recess and the further electrode and monitoring an electrical signal developed between the electrode in the recess and the further electrode.
30. An apparatus for supporting a layer separating two volumes of aqueous solution, the apparatus comprising:
elements defining a chamber, the elements including a body of non-conductive material having formed therein at least one recess opening into the chamber; and
an electrode contained in the recess.
31. An apparatus according to claim 30 , wherein surfaces including either or both of (a) the outermost surface of the body around the recess, and (b) at least an outer part of the internal surface of the recess extending from the rim of the recess, are hydrophobic.
32. An apparatus according to claim 31 , wherein the body comprises an outermost layer formed of a hydrophobic material, the recess extending through the outermost layer and said outer part of the internal surface of the recess being a surface of the outermost layer.
33. An apparatus according to claim 31 , wherein an inner part of the internal surface of the recess inside the outer part is hydrophilic.
34.-37. (canceled)
38. An apparatus according to claim 30 , wherein the body comprises a substrate and at least one further layer attached to the substrate, the recess extending through the at least one further layer.
39.-43. (canceled)
44. An apparatus according to claim 30 , wherein the electrode has provided thereon a hydrophillic surface which repels the hydrophobic fluid applied in step (c) whilst allowing ionic conduction from the aqueous solution to the electrode.
45.-47. (canceled)
48. An apparatus according to claim 30 , further comprising a further electrode in the chamber outside said recess.
49. An apparatus according to claim 30 , wherein the elements defining the chamber further include a cover extending over the body so that the chamber is a closed chamber, the cover comprising at least one inlet and at least one outlet.
50. (canceled)
51. An apparatus according to claim 30 , wherein the internal surface of the recess has no openings capable of fluid communication.
52.-56. (canceled)
57. An apparatus according to claim 30 , further comprising a pre-treatment coating of a hydrophobic fluid applied to the body across the recess.
58.-71. (canceled)
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STCB | Information on status: application discontinuation |
Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION |