IE84897B1 - A microfluidic analysis system - Google Patents
A microfluidic analysis systemInfo
- Publication number
- IE84897B1 IE84897B1 IE2007/0073A IE20070073A IE84897B1 IE 84897 B1 IE84897 B1 IE 84897B1 IE 2007/0073 A IE2007/0073 A IE 2007/0073A IE 20070073 A IE20070073 A IE 20070073A IE 84897 B1 IE84897 B1 IE 84897B1
- Authority
- IE
- Ireland
- Prior art keywords
- analysis system
- microfluidic analysis
- thermal
- detection
- conduit
- Prior art date
Links
- 238000004458 analytical method Methods 0.000 title claims description 31
- 238000001514 detection method Methods 0.000 claims abstract description 72
- 238000005382 thermal cycling Methods 0.000 claims abstract description 23
- 210000001736 Capillaries Anatomy 0.000 claims abstract description 12
- 238000004925 denaturation Methods 0.000 claims description 9
- 230000036425 denaturation Effects 0.000 claims description 9
- 238000001914 filtration Methods 0.000 claims description 9
- 238000005286 illumination Methods 0.000 claims description 7
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- 125000004122 cyclic group Chemical group 0.000 claims description 2
- 230000005670 electromagnetic radiation Effects 0.000 claims description 2
- 239000007788 liquid Substances 0.000 claims description 2
- 239000000523 sample Substances 0.000 description 59
- 230000003321 amplification Effects 0.000 description 24
- 238000003199 nucleic acid amplification method Methods 0.000 description 24
- 238000006243 chemical reaction Methods 0.000 description 19
- 238000000034 method Methods 0.000 description 17
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- 238000003753 real-time PCR Methods 0.000 description 10
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Abstract
ABSTRACT A thermal cycling device (3) device a number of fixed thermal zones (ll, 12, 13) and a fixed conduit (10) passing through the thermal zones. A controller maintains each thermal zone including its section of conduit (10) at a constant temperature. A series of droplets flows through the conduit (10) so that each droplet is thermally cycled, and a detection system detects fluorescence from droplets at all of the theimal cycles. The conduit is in a single plane, and so a number of thermal cycling devices may be arranged together to achieve parallelism. The flow conduit comprises a channel (17) and a capillary tube (10) inserted into the channel. The detection system may perform scans along a direction to detect radiation from a plurality of cycles in a pass.
Description
A Microfluidic Analysis Svstem
INTRODUCTION
Field of the Invention
The invention relates to analysis of samples to which thermal cycling is applied for
nucleic acid amplification, such as in the quantitative polymerase chain reaction
(qPCR).
Prior Art Discussion
Conventionally, nucleic acid amplification has involved providing an array of samples
in an assay plate and thermally cycling the plate reaction vessel. This, however,
involves the laborious task of loading the samples and preparing a fresh assay well
plate.
It is known to provide a thermal cycler for nucleic acid amplification, and
US5270l83, WO2005/075683, US6033880, and US6814934 describe thermal cycler
analysis systems.
The prior systems suffer from being complex, both in physical and control terms. For
example, in the system of US6033880 it is necessary to rotate heat exchangers into
desired positions, and in the system of US68l4934 it is necessary to heat and cool a
reaction vessel.
The invention is directed towards providing an improved thermal cycler system in
which a requirement to heat and cool a reaction vessel is avoided. Another object is to
achieve improved detection efficiency.
SUMMARY OF THE INVENTION
According to the invention, there is provided a microfluidic analysis system
comprising a thermal cycling device, the device having a plurality of fixed thermal
zones and a fixed conduit passing through the thermal zones, a controller for
maintaining each thermal zone including its section of conduit at a constant
temperature, means for flowing a series of droplets through the conduit so that each
droplet is thermally cycled, and a detection system for detecting electromagnetic
radiation from droplets at a plurality of said thennal cycles;
wherein the detection system performs simultaneous detection of emitted
radiation from a plurality of cycles;
wherein the flow conduit comprises a channel and a capillary tube inserted into
the channel; and
wherein the conduit is in a serpentine pattern of multiple folds, each fold
extending through a plurality of thermal zones.
In one embodiment, the conduit is in a single plane.
In another embodiment, the thermal zones are mutually thennally insulated.
In a further embodiment, the capillary has a circular cross-section.
In one embodiment, the channel and capillary are configured to receive a refractive
index—matching liquid in the channel and at least partly surrounding the capillary.
In another embodiment, the channel has a depth greater than that of the capillary.
In a further embodiment, the detection system comprises optics for filtering incident
radiation.
In one embodiment, the detection system comprises optics for filtering emitted
radiation.
In another embodiment, there is an air gap between adjacent thermal zones.
In a further embodiment, said air gap is adjustable.
In one embodiment, the flow conduit passes through a hot thermal zone for a length
before a first cycle, providing a denaturation zone.
In another embodiment, the detection system comprises a plurality of optic fibres for
point illumination of each of a plurality of cycles.
In a further embodiment, the detection system comprises a plurality of optic fibres for
point detection of each of a plurality of cycles.
In one embodiment, the detection system comprises a rotating filter for cyclic filtering
ofincident or emitted light.
In another embodiment, the system comprises a plurality of thermal cycling devices
arranged in parallel.
In a further embodiment, the thermal cycling devices are interconnected to form a
physical unit.
In one embodiment, the detection system performs simultaneous detection of emitted
light from a plurality of cycles fi'om a plurality of thermal cycling devices.
DETAILED DESCRIPTION OF THE INVENTION
Brief Description of the Drawings
The invention will be more clearly understood from the following description of some
embodiments thereof, given by way of example only with reference to the
aceompanyin g drawings in which:—
Fig. 1 is a block diagram of an analysis system of the invention;
Fig. 2 is a plan View of a thermal cycler of the system having three thermal
zones, Fig. 3 is a vertical cross section, and Fig. 4 is an end view of the thermal
cycler;
Fig. 5 is a perspective view of an alternative thermal cycler, having only two
thermal zones;
Fig. 6 is a diagram showing an arrangement with two exits, providing a choice
of 11 cycles or n+p cycles;
Fig. 7 is a photograph showing droplets flowing in a number of cycles of the
thermal cycler having three thermal zones;
Fig. 8 is a plot illustrating fluorescence characteristics for detection;
Fig. 9 is a block diagram of a detection system of the analysis system;
Fig. 10 is a pair of photographs, showing negative and positive fluorescence
detection, from lefi to right;
Figs. 11 to 14 are diagrams showing alternative detection arrangements;
Figs. 15 and 16 are perspective views showing image capture via optic fibres;
Fig. l7 is a perspective view of a three-dimensional cycler for parallel
amplification, and Fig. 18 is a cross-sectional plan view of this cycler;
Fig. 19 is a sample image of part of a detector array captured from the thermal
cycler of Fig. 17; and
Figs. 20 and 21 are views of arrays of windows of the cycler of Fig. 17.
Description of the Embodiments
An analysis system of the invention is based on microfluidics technology.
Microfluidic devices themselves have dimensions ranging from several millimetres to
micrometers. Typically one of the components or dimensions of the device, such as a
channel in the device, is of the order of micrometers.
The polymerase chain reaction, or PCR, is a powerfial technique used to amplify low
concentrations of specific DNA sequences to levels which may be detected. PC R can
be used to achieve a billionfold increase in target sequence copy number by thermally
cycling a specific chemical mix. This makes the PCR method extremely sensitive as it
can detect a single DNA molecule in a sample.
Fig. 1 shows an analysis system 1 for PCR. It has a sample preparation stage 2, a
thermal cycling stage 3 for PCR, a waste outlet 4, and a real time detection stage 5 to
achieve qPCR.
Fig. 2 shows the thermal cycler 3. It has a planar two dimensional serpentine channel
which is machined into a block which is segmented into three thermal zones 11,
12, and 13 separated by lmm air gaps 15. The three thermal zones are controlled to
achieve the three individual temperature zones required for the PCR reaction. Each
thermal section is controlled by continuous temperature sensing and a PID feedback
control system. Circular tubing is laid into a channel in a block of Al material to
ensure biocompatibility for the reaction. The circular tubing gives a smooth internal
surface and has no sharp edges to restrict the reaction. This results in stable, spherical
sample droplets. The tubing is embedded in the machined channel which results in
high heat transfer from the block to the sample.
Fig. 3 shows the machined channel 17 which contains the tubing 10 and a refractive
index matching solution. The machined channel 17 enables the introduction of the
refractive index matching solution 16 as it is considerably deeper than the diameter of
the tubing 10. The solution 16 covers the remainder of the channel above the tubing
and results in high accuracy detection through the tubing. An example of the
refractive index matching with the tubing is the use of a glycerine dilution solution.
The device is planar in design, which provides the ability for continuous detection
throughout the thermal cycling process. This enables real time quantitative detection
(termed “qPCR"). The assembly may be sealed using optical quality glass or thin film
adhesive.
Fig 4 shows thermal foil heaters 18 for heating the blocks of the thennal zones 11 and
13. The low temperature thermal zone 12 has a water channel 19 for maintaining a
unifonn low temperature. The thermal sections are controlled by temperature sensor
monitoring and a PID feedback control system.
The inlet to the analysis system 1 is connected to the PCR preparation system 2.
During sample preparation the double-stranded DNA sample is combined with two
oligonucleotide primers. The sample is segmented into droplets which are wrapped in
immiscible oil. The oil avoids cross contamination between the sequential droplets
and carry—over contamination within the device. This configuration avoids the need to
purge the system between different samples. A queue of different droplets from the
preparation system may be passed through the thermal cycler 3 directly. The block
and tubing are stationary so only the wrapped samples and oil solution move in the
thennal cycle system. Each thermal zone 11, 12, and 13, including the A1 block and
the embedded tubing 10, is an isothermal zone. Each zone is controlled to be
isothermal with respect to time. The velocity of the sample through the device is
defined by the control of the velocity of the carrier fluid. This is controlled by an
external pumping system. The velocity may then be varied to control the residency
time of the sample in each temperature zone 11-13.
The sample passes to the PCR thermal cycler 3 within the carrier fluid and through an
initial denaturation zone ll(a) before commencement of thermal cycling. The sample
passes into the high thermal section 11(a) where it is first separated into single
stranded DNA in a process called denaturation at a temperature TH.
The sample flows through the device at a steady controlled velocity to the second
temperature TL, where the hybridisation process takes place, during which the primers
anneal to the complementary sequences of the sample. Finally, as the sample flows
through the third and medium temperature zone, TM, the polymerase process occurs
when the primers are extended along the single strand of DNA with a thermostable
enzyme. The sample undergoes the same thermal cycling and chemical reaction as it
passes through N amplification cycles of the complete thermal device. This results in a
maximum two-fold amplification after each cycle and a total amplification of
I(1+E)N
where I is the initial product, E is the efficiency of the reaction and N is the number of
cycles.
Example
Fluorescent probes are contained in each sample droplet. The fluorescence level is
detected in each droplet at each cycle. This quantitative analysis provides information
on the specific concentration in the sample.
The three thermal zones are controlled to have temperatures as follows:
Zone ll 95°C (TH),
Zone 12 55°C (TL),
Zone 13 72°C (M).
The prepared sample droplets, wrapped in the carrier fluid, enter the inlet to the
thermal cycler at the controlled velocity. The sample then passes to the PCR thermal
cycler 3 within the carrier fluid and through the initial denaturation zone 1l(a) before
thermal cycling. The initial preheat is an extended zone to ensure the sample has
denatured successfully before thermal cycling. The requirement for a preheat zone and
the length of denaturation time required is dependent on the chemistry being used in
the reaction. The samples pass into the high temperature zone, of approximately 95°C,
where the sample is first separated into single stranded DNA in a process called
denaturation. The sample then flows to the low temperature zone 12, of approximately
55°C, where the hybridisation process takes place, during which the primers anneal to
the complementary sequences of the sample. Finally, as the sample flows through the
third medium temperature zone 13, of approximately 72°C, the polymerase process
occurs when the primers are extended along the single strand of DNA with a
thennostable enzyme. The sample undergoes the same thermal cycling and chemical
reaction as it passes through each thermal cycle of the serpentine pattern. The total
number of cycles in the device is easily altered by an extension of block length and
tubing. The system 1 has a total cycle number of 30 in this embodiment. The device
may be extended to a longer thermal cycler or a combination of two thermal cyclers to
achieve a greater cycle number.
Referring to Fig. 5, in a cycler 20 there are two temperature zones 21 and 23,
separated by an insulated air gap 24 to provide the correct temperatures zones
necessary for the PCR reaction. The zone 21 is heated by a thermal foil heater 22, and
the zone 23 is heated by natural convection from the top block 21. Again, the two
zones including the embedded tubing are stationary throughout the reaction and hence
isothermal with respect to time.
The section temperatures are:
Zone 21, 95°C (TH),
Zone 23, 60°C (T1),
The position of the lower block may be adjusted by increasing the insulation gap 24.
This adjusts the temperature of the zone 23. The tubing protrudes below the edge of
the bottom aluminium block when it is laid in the channel, providing an inspection
window. This is advantageous for the quantitative detection as it provides optical
access to the tubing in two planes.
The prepared sample droplets, wrapped in the carrier fluid, enter the inlet to the
thermal cycler at the controlled velocity. Different droplets are queued in the sample
preparation device and flow into the thermal cycler in a queue of droplets. A
suggested optimum configuration for droplet stability, and to avoid contamination, is a
droplet diameter of approximately 400nm, and a spacing of the same distance. The
wrapped nature of the droplets enables continuous flow of alternative droplets without
any contamination. This also removes the requirement to purge the system after each
reaction. The sample then passes to the PCR thermal cycler within the carrier fluid
and through an initial preheat zone before entering the thermal cycling. The preheat
zone is necessary for some chemistry for activation and also to ensure the sample is
fully denatured before the thermal cycling reaction begins. The preheat dwell length
results in approximately 10 minutes preheat of the droplets at the higher temperature.
The sample continues into the high temperature zone, of approximately 95°C, where
the sample is first separated into single stranded DNA in a process called denaturation.
The sample then flows through the device to the low temperature zone, of
approximately 60°C, where the hybridisation process takes place, during which the
primers anneal to the complementary sequences of the sample. Finally the polymerase
process occurs when the primers are extended along the single strand of DNA with a
thermostable enzyme. The sample undergoes the same thermal cycling and chemical
reaction as it passes through each thermal cycle of the complete device. The total
number of cycles in the device is easily altered by an extension of block length and
tubing. The system has a total cycle number of 50 in this embodiment. The device
may be extended to a longer thermal cycler or a combination of two thermal cyclers to
achieve a greater cycle number. Real time detection is applied to the device to provide
quantitative polymerase chain reaction (qPCR). This involves the use of fluorescent
probes such as SYBR Green or Taqman probes.
For a larger cycle number, or an optional extension to the cycle number, the device
may be divided into two sections; one with n cycles and one with p cycles as shown in
Fig. 6. The combination of the two devices enables a PCR total cycle number of n, p
or (n+p) depending on the tubing configuration and the heater control. Each block
may be separately controlled to allow for individual use or combined use. Therefore,
the cycle number of the device may be varied for greater versatility.
Case 1: Block 2 is thermally controlled and block 1 is uncontrolled (no
temperature input). The sample may then enter block 1, flow through the device
and exit the thermal cycler at exit 2 following p cycles.
Case 2: The two blocks are thermally controlled. Then the sample enters block
1, flows through the device and exits at exit 2 after (n+p) cycles.
Case 3: The tubing is changed to use exit 1. The sample enters block 1, flows
through block 1 and then exits at exit 1 following 11 cycles.
Fig. 7 shows a photograph of segmented droplets flowing though the thermal cycler
shown in Fig.2. The system allows for the quadruplicate amplification of a sample.
The design avoids cross contamination between successive samples and the planar
device allows full field detection during the thermal cycling.
A suggested optimum configuration for droplet stability, and to avoid contamination,
is a droplet diameter of approximately 400nm and a spacing of the same distance.
This configuration is suggested for the tubing used in this embodiment which has an
internal diameter of 400 pm. The wrapped nature of the droplets enables continuous
flow of alternative droplets without any contamination. This also removes the
requirement to purge the system.
Detection System
Quantitative PCR, or Q-PCR, is a variant of the basic PCR technique. The present Q-
PCR methods use fluorescent probes to monitor the amplification process as it
progresses. The SYBR Green I dye is commonly used for the fluorescent detection of
double-stranded DNA generated during PCR. The dye exhibits a peak excitation
maximum at 497 nm and a peak emission maximum at 520 nm. Taqman probes may
also be used which are a more target specific probe. The Taqman probes have
different excitation and emission wavelengths but one example is the F AM labelled
probe which has a peak excitation of 488nm and an emission of 520nm.
Through the analysis of the cycle-to-cycle change in fluorescence signal important
information regarding the DNA sample may be obtained. This is done by illuminating
the sample and detecting the resulting fluorescence. Different product concentration
will demonstrate fluorescence amplification at difference cycle numbers. Through the
analysis of the behaviour of the sample the characterisation is possible.
Fig 8 demonstrates an example of a fluorescence amplification curve. This was
demonstrated using a Taqman probe. There is little change in the fluorescent signal
after the first number of thermal cycles. This defines the baseline for the amplification
plot. Fluorescence intensity levels above this baseline represent amplification of PCR
product. A fluorescent threshold can be fixed above this baseline that defines the
threshold cycle, or Ct, for each reaction. The threshold cycle is defined as the
fractional cycle number at which the fluorescence passes above a fixed threshold. Ct is
observed in the early exponential stages of amplification. The higher the starting DNA
template concentration, the sooner a significant increase in fluorescence is observed.
Therefore the starting DNA concentration may be determined by the real time
fluorescent detection of the amplifying sample.
Referring to Fig. 9 the detection system 5 comprises:
, light source;
, optics for focusing the incident light;
, filters for filtering the incident light;
, focusing optics for focusing fluorescence emitted by the sample;
, filter optics for filtering the emitted fluorescence;
, sensor electronics; and
, processing electronics.
The choice of light source is dependent on the remainder of the detection system but
there are many options including filtered white light, specific wavelength laser or laser
diode. Fibre optics may also be incorporated for light transport. The filtering is
dependent on the light source and detection system but commercially available filter
components may be used.
If a detection indicator is used this will be provided in the sample preparation system.
The use of SYBR green fluorescence is demonstrated in Fig. 10. This demonstrates
the use of the fluorescence for the amplification detection in the tubing used in the
thermal cycler. The increase of fluorescence with increased sample amplification may
be seen from the images.
The detection sensor used is dependent on the field of view required and the
illumination wavelength chosen. Detector options include CCD, CMOS, photodiode
and photomultipliers
As the choice and combination of elements chosen are dependent on the overall
detection system design and implementation a number of systems are outlined below.
In summary, the system amplifies a DNA sample in a polymerase chain reaction
comprising the following steps:
a. Introducing spherical droplets of sample contained in an immiscible carrier
fluid to the thermal cycler
b. Passing the sample through circular tubing to provide a smooth internal surface
and no sharp edges allowing for most stable, spherical droplets.
c. Controlling the three thermal zones for successful reaction
d. Controlling the carrier fluid velocity by an external pumping system to achieve
the target residency times in the thermal zones
e. Passing the sample through the (three) thermally controlled zones to
successfully achieve DNA sample amplification.
f. Repeating step e the necessary number of times to achieve the desired sample
amplification
g. The quantitative detection of the amplification process.
The device is planar in design, enabling continuous quantitative PCR and multiple
levels for any desired level of parallelism.
The channel design enables manipulation for refiactive index matching within the
device for high quality detection. Also, the channel design results in high heat transfer
efficiency by embedding the tubing within the channel. As the droplets are wrapped in
an immiscible oil, sequential sample contamination or cross-over contamination
within the device is avoided.
Each thermal zone is controlled by continuous temperature sensing and a PID
feedback control system. In the embodiments there are 30 cycles and the particular
temperatures defined achieved successful denaturation, annealing and hybridisation
reactions.
Fig. 11 shows a full field detection system 40 which allows real time detection
without any moving parts. The system 40 comprises an illuminator 41 and lenses 42
illuminating the cycler 20, and a filter 43 for impingement of emission onto a detector
44. This enables global measurement of the full thermal cycler 20 or the specific
measurement at localised points along the thermal cycler. This is demonstrated in a
view of the detection system in Fig.l2, in which individual measurements are taken
for a linear series of points P. The detection measurement point in each cycle is
dependent on the fluorescent probes used for qPCR. Some probes fluoresce at any
point in the reaction whilst others only fluoresce at the annealing/extension stage.
Figs. 13 and 14 are scanning detection systems for two alternative configurations.
These systems also allow real time detection by moving the relative positions of the
detection system and the thermal cycler. In the system of Fig. 13 a positioning stage
45 moves the cycler 20, whereas in the system of Fig. 14 a positioning system 46
moves the illuminator 41 and the detector 44.
Whilst the above describes a single thermal cycler, the same movement may be
applied to multiple thermal cyclers by simple adding detection and illumination
points. The angle of illumination and detection, or orientation of the optical fibers.
may also be altered to facilitate multiple thermal cycler real time detection.
Figs. 15 and 16 show another quantitative detection configuration, 50. Optical fibers
are placed at each loop of the tubing in the block. A set of fibers 51 are placed
vertically below the thermal cycler 20 and the fiber ends are perpendicular to the
tubing. This bundle is attached to a light source 52 which excites the fluorescent
particles contained in the droplets as they pass the fiber ends. Another bundle of
fibers, 53, are placed horizontally at the front of the thermal cycler with the fiber ends
perpendicular to the tubing. This fiber bundle 53 collects the emitted light from the
fluorescent particles in the droplet as they pass the fiber ends. The other end of the
fiber bundle is detected by a camera 54 for detection of the droplet fluorescence. An
example of a detected fiber array is shown in Fig. 19. The continuous acquisition of
the fiber bundle image provides the quantitative detection of droplet fluorescence at
each individual fiber position. A filter wheel 55 may be used for alternative detection
of different fluorescent probes. For example, there are probes with excitation
wavelengths which are appropriate to use the same excitation source. However,
different detection bandwidths will enable the detection of different probes
individually. A filter wheel, a spectrometer or an alternative method of wavelength
separation will successfully achieve this goal.
Referring to Figs. 17 and 18, the throughput may also be increased by operating a
bank 60 of thermal cyclers 61 -64 in parallel. A planar system can achieve series
sampling of w samples and the parallel configuration can contain y parallel levels. The
continuous multi layered thermal cycler 60 results in the product (w x y) sample
capability. Such a PCR test of the whole genome of any living form, including the
human, could be addressed, which would have applications beyond diagnosis, in many
fields of pure and applied science. Fig. 18 shows a part of a cross-section through the
cycler, in the direction of the arrows XIX-XIX of Fig. 17. This shows the blocks 66
and 67 and the tubing 68. The tubing where it is exposed provides an array of
inspection windows 69.
All detection techniques may be applied to a multiple thermal cycler system for
quantitative detection. The protruding tubing array for a multiple thermal cycler
system, as shown in Fig. 17, can be seen in Fig. 20. Fig. 20 shows inspection windows
69 for a full 4 x 50 cycle system and Fig. 21 shows a detailed view of a small array of
inspection windows 69 more closely. The measurement points may be illuminated by
full field illumination or point illumination by high speed scarming or fiber optics. The
detection may be carried out the same way, by full field, scanning or simultaneous
point detection.
The invention improves upon current well based technology for the quantitative
amplification of nucleic acids. In that technology the reagents and sample are loaded
into a multi-well plate that is then thermally cycled, with each cycle approximately
number. The resulting fluorescent intensity increases
doubling the target
proportionally so that, with calibration, the amplification can be monitored with time.
Standard techniques are then available to calculate the number of targets initially
present, which is the required output for qPCR.
In this invention the data set is again three dimensional, monitoring over the x, y plane
and with time. The advantage over the well plate is that when plate amplification is
complete the plate must be cleaned or disposed with, and a new plate primed and
loaded onto the thermal cycling plate. In the invention the data is provided
continuously for as long as droplets are fed into the thermal cycler. Because there is
no carryover the system can be used continuously.
The geometric arrangement of the capillary tubing in the thermal cycler allows for
serial processing, a procession of droplets, parallel processing and an array of closely
packed capillary tubes. The rate of production of data is dependant upon the following
factors:
. The droplet length (c. 0.5mm)
. The droplet spacing (c. 1.5mm)
3. The droplet velocity (c. lmm/s)
4. The number of parallel lines.
Typical values are given in brackets. The possible degree of parallelism is very great.
Using 0.8mm outside diameter tubing, 100 parallel lines could only take up 80mm of
transverse width.
Using data above, following the time when the first droplets have completed
amplification, the system will produce an amplification curve every 0.02 seconds. or
180,000 curves per hour. This is far greater than anything available. Typical high-end
systems at present with 384 well plates would need to process 469 plates to achieve
the same data set.
The following are some applications of the invention:
— Rare target detection
— Multiple assay analysis
— Multiple sample/assay analysis
— End point qualitative detection
The invention is not limited to the embodiments described but may be varied in
construction and detail. For example, the overall pattern of the flow conduit may not
be serpentine. Alternatively, the thermal zones may be thennally controlled by flow of
hot water rather than directly by heaters in the hotter zones. Also, a thermoelectric
cooler may be used for one or more cooler zones. Further, the flow conduit may not be
in a repeated pattem. Instead, it may be straight or curved, passing through a plurality
of sets of thermal zones to provide cycles. Also, the detection may not involve
fluorescence detection. It may altematively involve detection of other parts of the
electromagnetic spectrum such as change of light polarisation, depending on the
desired detection technology.
Claims (1)
- Claims A microfluidic analysis system comprising a thermal cycling device, the device having a plurality of fixed thermal zones and a fixed conduit passing through the thermal zones, a controller for maintaining each thermal zone including its section of conduit at a constant temperature, means for flowing a series of droplets through the conduit so that each droplet is thermally cycled, and a detection system for detecting electromagnetic radiation from droplets at a plurality of said thennal cycles; wherein the detection system performs simultaneous detection of emitted radiation from a plurality of cycles; wherein the flow conduit comprises a channel and a capillary tube inserted into the channel; and wherein the conduit is in a serpentine pattem of multiple folds, each fold extending through a plurality of thermal zones. A microfluidic analysis system as claimed in claim 1, wherein the conduit is in a single plane. A microfluidic analysis system as claimed in claims 1 or 2, wherein the thermal zones are mutually thennally insulated. A microfluidic analysis system as claimed in any preceding claim, wherein the capillary has a circular cross—section. A microfluidic analysis system as claimed in any preceding claim, wherein the channel and capillary are configured to receive a refractive index-matching liquid in the channel and at least partly surrounding the capillary. A microfluidic analysis system as claimed in claim 5, wherein the charmel has a depth greater than that of the capillary. A microfluidic analysis system as claimed in any preceding claim, wherein the detection system comprises optics for filtering incident radiation. A microfluidic analysis system as claimed in any preceding claim, wherein the detection system comprises optics for filtering emitted radiation. A microfluidic analysis system as claimed in any preceding claim, wherein there is an air gap between adjacent thermal zones. A microfluidic analysis system as claimed in claim 9, wherein said air gap is adjustable. A microfluidic analysis system as claimed in any preceding claim, wherein the flow conduit passes through a hot thermal zone for a length before a first cycle, providing a denaturation zone. A microfluidic analysis system as claimed in any preceding claim, wherein the detection system comprises a plurality of optic fibres for point illumination of each of a plurality of cycles. A microfluidic analysis system as claimed in any preceding claim, wherein the detection system comprises a plurality of optic fibres for point detection of each of a plurality of cycles. A microfluidic analysis system as claimed in claims 12 or 13, wherein the detection system comprises a rotating filter for cyclic filtering of incident or emitted light. A microfluidic analysis system as claimed in any preceding claim, wherein the system comprises a plurality of thermal cycling devices arranged in parallel. A microfluidic analysis system as claimed in claim 15, wherein the thermal cycling devices are interconnected to form a physical unit. A microfluidic analysis system as claimed in claims 15 or 16 wherein the detection system performs simultaneous detection of emitted light from a plurality of cycles from a plurality of thermal cycling devices.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| IE2007/0073A IE84897B1 (en) | 2007-02-07 | A microfluidic analysis system |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| IEIRELAND07/02/20062006/0075 | |||
| IE20060075 | 2006-02-07 | ||
| IE2007/0073A IE84897B1 (en) | 2007-02-07 | A microfluidic analysis system |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| IE20070073A1 IE20070073A1 (en) | 2007-10-03 |
| IE84897B1 true IE84897B1 (en) | 2008-06-11 |
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