WO2017119382A1 - 反応処理装置、反応処理容器および反応処理方法 - Google Patents
反応処理装置、反応処理容器および反応処理方法 Download PDFInfo
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- B01L7/00—Heating or cooling apparatus; Heat insulating devices
- B01L7/52—Heating or cooling apparatus; Heat insulating devices with provision for submitting samples to a predetermined sequence of different temperatures, e.g. for treating nucleic acid samples
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- B01L3/50—Containers for the purpose of retaining a material to be analysed, e.g. test tubes
- B01L3/502—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
- B01L3/5027—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
- 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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- B01L3/502—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
- B01L3/5027—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
- B01L3/502746—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 for controlling flow resistance, e.g. flow controllers, baffles
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- B01L7/52—Heating or cooling apparatus; Heat insulating devices with provision for submitting samples to a predetermined sequence of different temperatures, e.g. for treating nucleic acid samples
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- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
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- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
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- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6806—Preparing nucleic acids for analysis, e.g. for polymerase chain reaction [PCR] assay
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/75—Systems in which material is subjected to a chemical reaction, the progress or the result of the reaction being investigated
- G01N21/77—Systems in which material is subjected to a chemical reaction, the progress or the result of the reaction being investigated by observing the effect on a chemical indicator
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- B01L2200/00—Solutions for specific problems relating to chemical or physical laboratory apparatus
- B01L2200/02—Adapting objects or devices to another
- B01L2200/026—Fluid interfacing between devices or objects, e.g. connectors, inlet details
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- B01L2200/10—Integrating sample preparation and analysis in single entity, e.g. lab-on-a-chip concept
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- B01L2300/08—Geometry, shape and general structure
- B01L2300/0809—Geometry, shape and general structure rectangular shaped
- B01L2300/0816—Cards, e.g. flat sample carriers usually with flow in two horizontal directions
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- B01L2300/0861—Configuration of multiple channels and/or chambers in a single devices
- B01L2300/0883—Serpentine channels
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- B01L2300/14—Means for pressure control
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- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0475—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure
- B01L2400/0481—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure squeezing of channels or chambers
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- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0475—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure
- B01L2400/0487—Moving fluids with specific forces or mechanical means specific mechanical means and fluid pressure fluid pressure, pneumatics
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- B—PERFORMING OPERATIONS; TRANSPORTING
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- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
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- B01L3/50—Containers for the purpose of retaining a material to be analysed, e.g. test tubes
- B01L3/502—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
- B01L3/5027—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
- B01L3/502715—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 interfacing components, e.g. fluidic, electrical, optical or mechanical interfaces
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- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
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- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6844—Nucleic acid amplification reactions
- C12Q1/686—Polymerase chain reaction [PCR]
Definitions
- the present invention relates to a reaction processing apparatus, a reaction processing container, and a reaction processing method used for polymerase chain reaction (PCR).
- PCR polymerase chain reaction
- Genetic testing is widely used for testing in various medical fields, identification of crops and pathogenic microorganisms, food safety assessment, and testing for pathogenic viruses and various infectious diseases.
- a method of analyzing a DNA obtained by amplifying a part of the DNA is known.
- PCR is a technique of attention that selectively amplifies a portion of a very small amount of DNA collected from a living body or the like.
- PCR is a specific part of DNA by applying a predetermined thermal cycle to a sample that is a mixture of a biological sample containing DNA and a PCR reagent composed of primers, enzymes, etc., and repeatedly causing reactions such as denaturation, annealing, and extension. Is selectively amplified.
- a reaction process that handles a very small amount of sample such as PCR is generally performed in a container called a vial or in a channel formed in a chip.
- a technique for performing PCR in the flow path may be advantageous, and many aspects thereof have been put into practical use.
- the thermal cycle of PCR it is necessary to repeat a temperature cycle from a low temperature of about 50 ° C. to a high temperature of about 95 ° C. a predetermined number of times for a sample in which DNA to be amplified and a PCR reagent are mixed. Since the sample is usually an aqueous solution, the vapor pressure increases in the 95 ° C. region, and the water component of the sample is likely to evaporate. If the water component of the sample evaporates, the concentration of the sample may increase, and parameters such as the optical characteristics of the sample may unexpectedly fluctuate, causing problems such as inability to properly manage the reaction process. .
- the atmospheric pressure decreases as the altitude increases, the boiling point significantly decreases in such an environment, and the sample is likely to boil.
- the atmospheric pressure is approximately 897 hPa and the boiling point is calculated to be 96.6 ° C.
- the atmospheric pressure is 845 hPa and the boiling point is 95 ° C
- the atmospheric pressure is 797 hPa and the boiling point. Is 93.4 ° C.
- the air pressure in the airliner is about 800 hPa, which is equivalent to an altitude of about 2000 m, and the boiling point is about 93 ° C., so that it is substantially difficult to perform PCR even in an aircraft in flight.
- Even on flat ground it is highly probable that the sample will partially evaporate even if it is not boiled by raising the temperature of the sample consisting mainly of an aqueous solution to around 95 ° C. May not be measured accurately.
- JP 2009-232700 A Japanese Patent Laid-Open No. 9-262084
- Patent Document 1 an operation of covering with a sample such as oil in a mode in which a sample to be subjected to PCR is sandwiched is very troublesome and the sample is prevented from being contaminated. There is also a problem from the point of view. Furthermore, in the aspect which concerns on patent document 1, it is thought that it may be unable to suppress that a sample boils in the environment where the boiling point of a sample becomes low.
- the present invention has been made in view of such circumstances, and its purpose is to provide a reaction processing apparatus, a reaction processing container, and a reaction capable of performing PCR while preventing the sample from boiling and generating bubbles even in a low atmospheric pressure location. It is to provide a processing method.
- a reaction processing apparatus includes a mounting unit for mounting a plate-like reaction processing container including a channel into which a sample is introduced, and a sample in the channel.
- a temperature control system that controls the temperature of the region where the flow path exists, and a liquid feeding system that controls the pressure in the flow path of the reaction processing container to move the sample in the flow path.
- the liquid feeding system maintains the pressure in the flow path during the reaction process of the sample higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus, preferably 1 atmosphere or more.
- the liquid feeding system includes a pressurizing chamber in which the internal pressure is higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus, and preferably maintained at 1 atm or higher, and a liquid feeding pump disposed in the pressurizing chamber. Also good.
- the output of the pump for feeding liquid and the first communication port provided at one end of the flow path of the reaction processing container are communicated, and the inside of the pressurization chamber and the other end of the flow path of the reaction processing container are provided. Two communication ports may be communicated.
- the reaction processing apparatus may further include a control unit that controls the liquid feeding pump in order to move the sample in the flow path.
- the liquid delivery system includes a pressurized chamber whose internal pressure is higher than the atmospheric pressure of the surrounding environment of the reaction processing apparatus, and preferably maintained at 1 atmosphere or higher, a first liquid delivery pump disposed in the pressurized chamber, And a second liquid feeding pump disposed in the pressurizing chamber.
- the output of the first liquid feed pump communicates with the first communication port provided at one end of the flow path of the reaction processing container, and the output of the second liquid feed pump and the other end of the flow path of the reaction processing container.
- the 2nd communicating port provided in may be connected.
- the reaction processing apparatus may further include a control unit that controls the first liquid feeding pump and the second liquid feeding pump in order to move the sample in the flow path.
- the liquid feeding system has a pressurized chamber in which the internal pressure is higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus, and preferably maintained at 1 atmosphere or more, and the internal pressure is maintained at a pressure higher than that in the pressurized chamber.
- a liquid feed chamber, a first direction switching valve for communicating one of the pressurization chamber and the liquid feed chamber with a first communication port provided at one end of a flow path of the reaction processing container, a pressurization chamber, and a liquid feed chamber You may provide the 2nd direction switching valve which connects any one of these to the 2nd communicating port provided in the other end of the flow path of the reaction processing container.
- the reaction processing apparatus may further include a control unit that controls the first direction switching valve and the second direction switching valve in order to move the sample in the flow path.
- Another aspect of the present invention is a reaction processing method.
- This method includes a step of placing a reaction container having a flow channel into which a sample is introduced, a step of controlling the temperature of the flow channel in order to heat the sample in the flow channel, and a sample in the flow channel. And a step of controlling the pressure in the flow path of the reaction processing container in order to move.
- the pressure in the flow path is higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus, and preferably maintained at 1 atmosphere or more.
- reaction processing apparatus capable of performing PCR while preventing boiling of a sample and generation of bubbles even at a low atmospheric pressure location.
- FIGS. 1A and 1B are diagrams for explaining a reaction processing container that can be used in the reaction processing apparatus according to the first embodiment of the present invention. It is a figure which shows typically a mode that the sample was introduce
- FIGS. 5A and 5B are diagrams for explaining a reaction processing container that can be used in the reaction processing apparatus according to the second embodiment of the present invention. It is a schematic diagram for demonstrating the reaction processing apparatus which concerns on 2nd Embodiment of this invention.
- reaction processing apparatus is an apparatus for performing PCR. It should be noted that the same or equivalent components, members, and processes shown in the drawings are denoted by the same reference numerals, and repeated descriptions are omitted as appropriate.
- the embodiments do not limit the invention but are exemplifications, and all features and combinations thereof described in the embodiments are not necessarily essential to the invention.
- FIGS. 1A and 1B are views for explaining a reaction processing container 10 that can be used in the reaction processing apparatus according to the first embodiment of the present invention.
- FIG. 1A is a plan view of the reaction processing container 10
- FIG. 1B is a front view of the reaction processing container 10.
- the reaction processing container 10 includes a substrate 14 and a flow path sealing film 16.
- the substrate 14 is preferably formed of a material that is stable against temperature changes and hardly corroded by the sample solution used. Furthermore, the substrate 14 is preferably formed of a material having good moldability, good transparency and barrier properties, and low autofluorescence. As such a material, not only inorganic materials such as glass and silicon (Si) but also resins such as acrylic, polyester, and silicone, among which cycloolefin is preferable.
- An example of the dimensions of the substrate 14 is a long side of 70 mm, a short side of 42 mm, and a thickness of 3 mm.
- a groove-like flow path 12 is formed on the lower surface 14 a of the substrate 14, and the flow path 12 is sealed with a flow path sealing film 16.
- the flow channel 12 is formed in a so-called meandering shape in which a curved portion (turn) and a straight portion are folded back in plan view. Specifically, a combination consisting of a pair of turn portions on both sides (corresponding to a high temperature region and a low temperature region described later) and two straight portions connecting them (corresponding to the medium temperature region) is taken as one unit and given to the sample. Consecutively configure units that are more than the expected number of thermal cycles.
- An example of the dimensions of the flow path 12 formed on the lower surface 14a of the substrate 14 is a width of 0.7 mm and a depth of 0.7 mm.
- a first communication port 17 communicating with the outside is formed at one end of the flow path 12 in the substrate 14.
- a second communication port 18 is formed at the other end of the flow path 12 in the substrate 14.
- a pair of first communication port 17 and second communication port 18 formed at both ends of the flow path 12 are formed so as to be exposed on the upper surface 14 b of the substrate 14.
- Such a substrate can be manufactured by injection molding or cutting by an NC processing machine.
- a flow path sealing film 16 is stuck on the lower surface 14a of the substrate 14.
- most of the flow path 12 is formed in a groove shape exposed on the lower surface 14 a of the substrate 14. This is to facilitate molding by injection molding using a mold or the like.
- a flow path sealing film 16 is pasted on the lower surface 14a of the substrate 14.
- the flow path sealing film 16 one main surface may be provided with adhesiveness, and a functional layer that exhibits adhesiveness and adhesiveness by pressing may be formed on one main surface, and easily. It has a function that can be integrated with the lower surface 14a of the substrate 14 in close contact.
- the channel sealing film 16 is preferably formed of a material having low autofluorescence including an adhesive.
- a transparent film made of a resin such as cycloolefin polymer, polyester, polypropylene, polyethylene, or acrylic is suitable, but not limited thereto.
- the flow path sealing film 16 may be formed from plate-shaped glass or resin. In this case, since a rigid property can be expected, it is useful for preventing warping and deformation of the reaction processing vessel 10.
- FIG. 2 schematically shows a state in which the sample 20 is introduced into the flow path 12 of the reaction processing vessel 10.
- the sample 20 is represented by a solid line thicker than the flow path 12 in order to emphasize the position of the sample 20. It should be noted that the sample 20 does not represent a state of protruding from the flow path.
- the sample 20 is introduced into the flow path 12 from either the first communication port 17 or the second communication port 18.
- the introduction method is not limited to these, but an appropriate amount of sample may be directly introduced from the communication port using, for example, a pipette, a dropper, or a syringe. Alternatively, it may be an introduction method while preventing contamination through a cone-shaped needle tip in which a filter made of porous PTFE or polyethylene is incorporated. In general, many types of such needle tips are sold and easily available, and can be used by being attached to the tip of a pipette, dropper, syringe or the like.
- the sample may be moved to a predetermined location in the flow path as shown in FIG.
- the initial position of the sample as shown in FIG. 4, an example in which a position in a high-temperature region 40 described later is set as the initial position is given, but the present invention is not limited to this.
- a mixture containing two or more types of DNA for example, to a mixture containing two or more types of DNA, a plurality of types of primers, a thermostable enzyme, and four types of deoxyribonucleoside triphosphates (dATP, dCTP, dGTP, dTTP) were added as PCR reagents. Things can be raised. Further, a fluorescent probe that reacts specifically with the DNA to be treated is mixed. Commercially available reagent kits for real-time PCR can also be used.
- dATP deoxyribonucleoside triphosphates
- FIG. 3 is a schematic diagram for explaining the reaction processing apparatus 30 according to the first embodiment of the present invention.
- FIG. 4 is a view for explaining a state in which the reaction processing container 10 is set at a predetermined position of the reaction processing apparatus 30.
- the reaction processing apparatus 30 includes a reaction processing container mounting portion (not shown) on which the reaction processing container 10 is mounted, a temperature control system 32, and a CPU.
- the temperature control system 32 has a region 40 approximately 1/3 below the paper surface in the flow path 12 of the reaction processing container 10 with respect to the reaction processing container 10 mounted on the reaction processing container mounting portion. Is approximately 95 ° C., the region 42 approximately 1/3 above the paper surface is approximately 55 ° C., and the region 1/3 in the middle of the paper surface is approximately 3 ° C. Yes.
- the region 40 of the flow channel 12 is appropriately referred to as “high temperature region 40”
- the region 41 of the flow channel 12 is referred to as “medium temperature region 41”
- the region 42 of the flow channel 12 is referred to as “low temperature region 42”. This is referred to as a thermal cycle region.
- the temperature control system 32 maintains the temperature of each temperature region in the thermal cycle region.
- the temperature control system 32 includes a high-temperature heater 60 for heating the high-temperature region 40 of the flow path 12, and the flow path 12.
- a medium temperature heater 61 for heating the medium temperature region 41, a low temperature heater 62 for heating the low temperature region 42 of the flow path 12, and a temperature sensor (such as a thermocouple) for measuring the actual temperature in each temperature region (Not shown)
- a high temperature heater driver 33 for controlling the temperature of the high temperature heater 60
- a medium temperature heater driver 34 for controlling the temperature of the medium temperature heater 61
- a low temperature heater for controlling the temperature of the low temperature heater 62
- the actual temperature information measured by the temperature sensor is sent to the CPU 36.
- each heater may be, for example, a resistance heating element or a Peltier element.
- the temperature control system 32 may further include other component parts for improving the temperature controllability of each temperature region.
- the reaction processing apparatus 30 further includes a liquid feeding system 37 for moving the sample 20 in the flow path 12 of the reaction processing container 10.
- a liquid feeding system 37 for moving the sample 20 in the flow path 12 of the reaction processing container 10.
- the sample 20 is continuously moved in one direction in the flow path 12, and each of the samples in the thermal cycle region of the reaction processing container 10 is moved.
- the temperature region can be passed, and as a result, the sample 20 can be given a thermal cycle. More specifically, by applying the steps of denaturation in the high temperature region 40, annealing in the low temperature region 42, and extension in the intermediate temperature region 41, the target DNA in the sample 20 is selectively amplified.
- the high temperature region 40 can be regarded as a denaturing temperature region, the low temperature region 42 as an annealing temperature region, and the intermediate temperature region 41 as an elongation temperature region.
- the residence time in each temperature region is the time for the sample to stop at a predetermined position in each temperature region, the moving speed of the sample, the size (area) of each temperature region, and the flow path length corresponding to each temperature region. It can be set appropriately by changing the above.
- the annealing temperature region and the elongation temperature region may be integrated to form an annealing / elongation temperature region. In this case, it becomes a thermal cycle region composed of two temperature regions, a high temperature region for modification and a lower temperature region (medium / low temperature region).
- the liquid feeding system 37 includes a pressurizing chamber 38, a liquid feeding pump 39, a liquid feeding pump driver 43 for controlling the liquid feeding pump 39, a pressure chamber pump 44, and the pressure chamber.
- a pressurizing chamber pump driver 45 for controlling the working pump 44, a first tube 46, and a second tube 47.
- the first end 46 a of the first tube 46 is connected to the first communication port 17 of the reaction processing container 10. It is preferable that a packing or a seal for ensuring airtightness is disposed at a connection portion between the first communication port 17 and the first end 46 a of the first tube 46.
- the second end 46 b of the first tube 46 is connected to the output of the liquid feed pump 39.
- the liquid feed pump 39 may be a micro blower pump composed of a diaphragm pump, for example.
- the CPU 36 controls the blowing and pressurization from the liquid feed pump 39 via the liquid feed pump driver 43.
- the blowing or pressurization from the liquid feed pump 39 acts on the sample 20 in the flow path 12 through the first communication port 17 and moves the sample 20 as a driving force.
- liquid feeding pump 39 for example, a micro blower pump (model MZB1001T02) manufactured by Murata Manufacturing Co., Ltd. can be used. This micro blower pump can increase the pressure on the secondary side from the primary side during operation, but the pressure on the primary side and the secondary side are equal at the moment of stopping or at the time of stopping.
- the liquid feeding pump 39 is entirely disposed in the pressurizing chamber 38.
- the first end 47 a of the second tube 47 is connected to the second communication port 18 of the reaction processing container 10. It is preferable that a packing or a seal for ensuring airtightness is disposed at a connection portion between the second communication port 18 and the first end 47 a of the second tube 47.
- the second end 47 b of the second tube 47 is connected so as to communicate with the pressurizing chamber 38. Thereby, the second communication port 18 of the reaction processing vessel 10 communicates with the atmosphere in the pressurization chamber 38.
- the pressurizing chamber 38 forms a space having a constant volume therein.
- a pressurizing chamber pump 44 is connected to the pressurizing chamber 38.
- the pressurizing chamber pump driver 45 controls the pressurizing chamber pump 44 according to an instruction from the CPU 36 so that the space in the pressurizing chamber 38 becomes a predetermined pressure.
- a small DC diaphragm pump (model DSA-1-12BL) manufactured by Denso Sangyo Co., Ltd. can be used. Means can also be used.
- the pressure in the pressurizing chamber 38 is set higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 30 during the reaction process, and more preferably maintained at 1 atm (1013 hPa) or more.
- the atmospheric pressure in the surrounding environment of the reaction processing apparatus refers to the place where the reaction processing apparatus according to the present invention is installed, the place where the reaction process is performed by the apparatus, or the place where the reaction processing apparatus is partitioned from the surroundings. Is the pressure (or atmospheric pressure) at the partitioned location.
- the pressure in the pressurizing chamber 38 should be high enough to prevent the sample from evaporating or generating bubbles that may affect the PCR reaction process even if the sample is repeatedly exposed to high temperatures (about 95 ° C.). Good.
- the higher the pressure in the pressurizing chamber 38 the more the influence of sample evaporation and the like can be suppressed.
- the liquid feeding system 37 is complicated and enlarged including its handling, a person skilled in the art Can comprehensively judge the use, purpose, cost, and effect of the device and design the entire system.
- the pressure chamber 38 is provided with an atmospheric pressure release valve 48.
- the atmospheric pressure release valve 48 is used when the reaction processing container 10 is attached to or detached from the reaction processing apparatus 30, such as the liquid feeding system 37 (inside the pressurization chamber 38, the first tube 46, the second tube 47, etc.)
- the pressure in the flow path 12 is controlled to be equal to the atmospheric pressure in the surrounding environment of the reaction processing apparatus 30. Thereby, the rapid movement and jumping out of the sample 20 can be prevented.
- the pressurizing chamber 38 may be provided with a pressure sensor (not shown) for constantly monitoring the pressure in the internal space. By sending the actual pressure detected by the pressure sensor to the CPU 36, the pressure in the pressurizing chamber 38 can be suitably controlled.
- the reaction processing apparatus 30 further includes a fluorescence detector 50.
- the fluorescence from the sample 20 in the flow path 12 of the reaction processing container 10 is detected using the fluorescence detector 50, and the value can be used as an index as a determination material for PCR progress or reaction termination.
- the fluorescence detector 50 an optical fiber type fluorescence detection manufactured by Nippon Sheet Glass Co., Ltd., which can measure rapidly with a very compact optical system and can detect fluorescence regardless of whether it is a bright place or a dark place.
- the instrument FLE-510 can be used.
- the wavelength characteristics of the excitation light / fluorescence can be tuned so as to be suitable for the fluorescence characteristics emitted by the sample 20, and an optimum optical / detection system for a sample having various characteristics can be obtained. It is possible to provide.
- the optical fiber type fluorescence detector 50 includes an optical head 51, a fluorescence detector driver 52, and an optical fiber 53 that connects the optical head 51 and the fluorescence detector driver 52.
- the fluorescence detector driver 52 includes an excitation light source (LED, laser or other light source adjusted to emit a specific wavelength), an optical fiber type multiplexer / demultiplexer, and a photoelectric conversion element (PD, APD, photomultiplier, etc.). Photo detector) (none of which are shown) and the like, and includes a driver for controlling them.
- the optical head 51 includes an optical system such as a lens, and has a function of directing the excitation light to the sample and condensing fluorescence emitted from the sample.
- the condensed fluorescence is separated from the excitation light by the optical fiber type multiplexer / demultiplexer in the fluorescence detector driver 52 through the optical fiber 53 and converted into an electric signal by the photoelectric conversion element.
- the optical head 51 may be disposed near the second communication port 18 of the reaction processing container 10. In this case, it is possible to know that the amplification of DNA has been completed by detecting the fluorescence from the sample 20 sent to the vicinity of the second communication port 18 after a series of reaction processes.
- a plurality of optical heads 51 may be arranged so as to detect fluorescence from the sample 20 in the vicinity of the first communication port 17 or in the midway flow path 12.
- the fluorescence detector is not limited to the optical fiber fluorescence detector as long as it exhibits a function of detecting fluorescence from the sample.
- a reaction processing method using the reaction processing apparatus 30 configured as described above will be described.
- the second end 46b of the first tube 46 is connected to the output of the liquid feed pump 39, and the first end 46a of the first tube 46 is open.
- the second end 47b of the second tube 47 is connected to the pressurizing chamber 38, and the first end 47a of the second tube 47 is open.
- the reaction processing container 10 is placed on the reaction processing container mounting portion of the reaction processing apparatus 30.
- the atmospheric pressure release valve 48 provided in the pressurizing chamber 38 is opened, and the first tube scheduled to be connected to the pressurizing chamber 38 and the first communication port 17 and the second communication port 18 of the reaction processing vessel 10. 46, the pressure in the second tube 47 is the same as the atmospheric pressure. Subsequently, the first end 46 a of the first tube 46 extending from the liquid feed pump 39 is connected to the first communication port 17 of the reaction processing vessel 10, and the first end of the second tube 47 extending from the pressurizing chamber 38. 47 a is connected to the second communication port 18 of the reaction processing vessel 10. Neither the liquid feed pump 39 nor the pressurizing chamber pump 44 is operated at this time. Subsequently, the atmospheric pressure release valve 48 provided in the pressurizing chamber 38 is closed.
- the pressurizing chamber pump 44 is operated, and the pressure of the flow path 12 in the pressurizing chamber 38 and the reaction processing vessel 10 communicating with the pressurizing chamber 38 is higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 30, preferably 1 atm. (1013 hPa) or more.
- the pressure on the primary side and the secondary side are equal, that is, the pressure of the first communication port 17 communicating with the secondary side of the liquid feed pump 39 is also increased. It is equal to the pressure in the chamber 38. Therefore, since the pressures in the spaces (the first communication port 17 side and the second communication port 18 side) on both sides of the sample 20 in the flow path 12 of the reaction processing container 10 are equal, the sample 20 does not move.
- the aqueous solution is mainly from an aqueous solution even in a low atmospheric pressure environment such as a high altitude. It is possible to prevent the sample 20 from boiling and foaming by lowering the boiling point of the sample 20.
- the liquid feed pump 39 is operated by the liquid feed pump driver 43. Accordingly, the pressure in the flow path 12 on the first communication port 17 side in the flow paths 12 on both sides of the sample 20 becomes higher than that on the second communication port 18 side. It can be moved in the direction of the flow path 12.
- the sample 20 passes through the continuous meandering flow path 12 through each temperature region of the denaturation region (high temperature region 40), the annealing region (low temperature region 42), and the extension region (medium temperature region 41) in a cyclic manner. .
- a reaction processing apparatus in which a two-level temperature region is set, it passes through each temperature region of the denaturation region (high temperature region) -annealing / extension region (medium / low temperature region) continuously in a cycle. Thereby, the sample 20 is given a predetermined number of thermal cycles, PCR occurs, and a predetermined DNA can be selectively amplified.
- the pressure in the flow path 12 of the reaction processing container 10 is always higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 30, preferably It is maintained at 1 atmosphere or more. That is, during the reaction process, the sample 20 is constantly pressurized to a pressure higher than the ambient pressure of the reaction processing apparatus 30, preferably 1 atmosphere or more. Therefore, PCR can be performed while preventing boiling of the sample and generation of bubbles even in places with low atmospheric pressure such as in high altitudes or in airplanes.
- FIGS. 5A and 5B are views for explaining a reaction processing vessel 110 that can be used in the reaction processing apparatus according to the second embodiment of the present invention.
- 5A is a plan view of the reaction processing container 110
- FIG. 5B is a front view of the reaction processing container 110.
- the reaction processing container 110 includes a substrate 114 and a flow path sealing film 116.
- the structure of the substrate 114 and the flow path sealing film 116 such as the material and dimensions is the same as that of the reaction processing container 10 described in the first embodiment.
- a groove-shaped channel 112 is formed on the lower surface 114 a of the substrate 114, and the channel 112 is sealed with a channel sealing film 116.
- An example of the dimensions of the flow path 112 formed on the lower surface 114a of the substrate 114 is a width of 0.7 mm and a depth of 0.7 mm.
- a first communication port 117 communicating with the outside is formed at one end of the flow path 112 in the substrate 114.
- a second communication port 118 is formed at the other end of the flow path 112 in the substrate 114.
- a pair of first communication ports 117 and second communication ports 118 formed at both ends of the flow path 112 are formed so as to be exposed on the upper surface 114 b of the substrate 114.
- a flow path sealing film 116 is attached on the lower surface 114a of the substrate 114.
- most of the flow path 112 is formed in a groove shape exposed on the lower surface 114 a of the substrate 114. This is because it can be easily formed by injection molding using a mold or the like or cutting by an NC processing machine. In order to seal this groove and use it as a flow path, a flow path sealing film 116 is stuck on the lower surface 114 a of the substrate 114.
- the reaction processing container 110 of the second embodiment includes a temperature region in which a plurality of levels of temperature control is possible in the flow path 112 between the pair of communication ports as in the reaction processing container 10 of the first embodiment.
- the difference from the reaction processing container 10 of the first embodiment is that the flow path 112 is not a so-called continuous meandering flow path.
- the sample is not sent in a one-way continuous flow to the meandering flow path that is continuously folded as in the reaction processing container 10 of the first embodiment, but a plurality of at least one flow path 112 is provided. This is because it is planned to feed the sample so as to continuously reciprocate between the temperature regions in which the standard temperature is maintained.
- the portion of the flow channel 112 corresponding to each temperature region in the flow channel 112 is composed of a curved portion (turn) and a straight portion within each temperature region (small compared to the first embodiment) in a meandering form.
- Each temperature region may be connected by a short flow path, for example. Since each temperature region can have a smaller area and channel length than that of the first embodiment, it is relatively easy to reduce temperature variations in each temperature region, and the entire channel length can be shortened. There is an advantage that the reaction processing container and the reaction processing apparatus can be made small.
- FIG. 6 is a schematic diagram for explaining a reaction processing apparatus 130 according to the second embodiment of the present invention.
- FIG. 7 is a diagram for explaining a state in which the reaction processing container 110 is set at a predetermined position of the reaction processing apparatus 130.
- the sample 120 is introduced into the flow path 112 of the reaction processing container 110.
- the sample 120 is represented by a solid line thicker than the flow path 112 in order to emphasize the position of the sample 120. It should be noted that the sample 120 does not represent a state of protruding from the flow path.
- the sample 120 and its introduction method are the same as those in the first embodiment.
- the initial position of the sample 120 as shown in FIG. 7, an example in which a position in a high-temperature region 140 described later is set as the initial position is given, but the present invention is not limited to this.
- the reaction processing apparatus 130 includes a reaction processing container mounting portion (not shown) on which the reaction processing container 110 is mounted, a temperature control system 132, and a CPU 136.
- the temperature control system 132 has a region 140 that is approximately 3 of the right side of the paper surface in the flow path 112 of the reaction processing container 110 with respect to the reaction processing container 110 mounted on the reaction processing container mounting portion. Is approximately 95 ° C., and the region 142 on the left side of the drawing is approximately 55 ° C., and the region 1/3 in the middle of the drawing is maintained and controlled at three levels of approximately 72 ° C. with high accuracy. Yes.
- the region 140 of the flow path 112 is appropriately referred to as a “high temperature region 140”
- the region 141 of the flow path 112 is referred to as an “intermediate temperature region 141”
- the region 142 of the flow path 112 is referred to as a “low temperature region 142”. This is referred to as a thermal cycle region.
- the temperature control system 132 maintains each temperature region of the thermal cycle region.
- the temperature control system 132 includes a high-temperature heater 160 for heating the high-temperature region 140 of the flow path 112, and an intermediate-temperature region of the flow path 112. 41, a medium temperature heater 161 for heating 41, a low temperature heater 162 for heating the low temperature region 40 of the flow path 112, and a temperature sensor (not shown) such as a thermocouple for measuring the actual temperature in each temperature region. 2), a high temperature heater driver 133 that controls the temperature of the high temperature heater 160, an intermediate temperature heater driver 134 that controls the temperature of the intermediate temperature heater 161, and a low temperature heater driver 135 that controls the temperature of the low temperature heater 162.
- a high temperature heater driver 133 that controls the temperature of the high temperature heater 160
- an intermediate temperature heater driver 134 that controls the temperature of the intermediate temperature heater 161
- a low temperature heater driver 135 that controls the temperature of the low temperature heater 162.
- the actual temperature information measured by the temperature sensor is sent to the CPU 136.
- the CPU 136 controls each heater driver based on the actual temperature information of each temperature region so that the temperature of each heater becomes a predetermined temperature.
- Each heater may be, for example, a resistance heating element or a Peltier element.
- the temperature control system 132 may further include other component parts for improving the temperature controllability of each temperature region.
- the reaction processing apparatus 130 further includes a liquid feeding system 137 for moving the sample 120 in the flow path 112 of the reaction processing container 110.
- a liquid feeding system 137 for moving the sample 120 in the flow path 112 of the reaction processing container 110.
- the sample 120 is continuously moved in a reciprocating manner in the flow path 112, and each temperature in the thermal cycle region of the reaction processing vessel 110 is changed.
- the region can be passed, so that the sample 120 can be given a thermal cycle. More specifically, by applying the steps of denaturation in the high temperature region 140, annealing in the low temperature region 142, and extension in the medium temperature region 141, the target DNA in the sample 120 is selectively amplified.
- the high temperature region 140 can be regarded as a denaturing temperature region
- the low temperature region 142 can be regarded as an annealing temperature region
- the intermediate temperature region 141 as an elongation temperature region.
- the residence time in each temperature region is the time for the sample to stop at a predetermined position in each temperature region, the moving speed of the sample, the size (area) of each temperature region, and the flow path length corresponding to each temperature region. It can be set appropriately by changing the above.
- the annealing temperature region and the elongation temperature region may be integrated to form an annealing / elongation temperature region. In this case, it becomes a thermal cycle region composed of two temperature regions, a high temperature region for modification and a lower temperature region (medium / low temperature region).
- the liquid feeding system 137 includes a pressurizing chamber 138, a first liquid feeding pump 139, a first liquid feeding pump driver 143 for controlling the first liquid feeding pump 139, and a second liquid feeding pump. 165, a second liquid feed pump driver 166 for controlling the second liquid feed pump 165, a pressurization chamber pump 144, and a pressurization chamber for controlling the pressurization chamber pump 144 A pump driver 145, a first tube 146, and a second tube 147 are provided.
- the first end 146 a of the first tube 146 is connected to the first communication port 117 of the reaction processing vessel 110. It is preferable that a packing or a seal for ensuring airtightness is disposed at a connection portion between the first communication port 117 and the first end 146a of the first tube 146.
- the second end 146b of the first tube 146 is connected to the output of the first liquid feeding pump 139.
- the first liquid feeding pump 139 may be a micro blower pump including a diaphragm pump, for example.
- the first end 147 a of the second tube 147 is connected to the second communication port 118 of the reaction processing vessel 110.
- a packing or a seal for ensuring airtightness is disposed at a connection portion between the second communication port 118 and the first end 147a of the second tube 147.
- the second end 147 b of the second tube 147 is connected to the output of the second liquid feeding pump 165.
- the second liquid feeding pump 165 may be a micro blower pump composed of a diaphragm pump, for example.
- the CPU 136 controls air blowing and pressurization from the first liquid feeding pump 139 and the second liquid feeding pump 165 via the first liquid feeding pump driver 143 and the second liquid feeding pump driver 166.
- the blowing and pressurization from the first liquid feeding pump 139 and the second liquid feeding pump 165 act on the sample 120 in the flow path 112 through the first communication port 117 and the second communication port 118, and become a driving force.
- the sample 120 is moved.
- first liquid feed pump 139 and the second liquid feed pump 165 for example, a micro blower pump (model MZB1001T02) manufactured by Murata Manufacturing Co., Ltd. can be used.
- both the first liquid feeding pump 139 and the second liquid feeding pump 165 are disposed in the pressurizing chamber 138 as a whole.
- the pressurizing chamber 138 forms a space having a constant volume therein.
- a pressurization chamber pump 144 is connected to the pressurization chamber 138.
- the pressurizing chamber pump driver 145 controls the pressurizing chamber pump 144 according to an instruction from the CPU 136 so that the space in the pressurizing chamber 138 becomes a predetermined pressure.
- a compact DC diaphragm pump (model DSA-1-12BL) manufactured by Denso Sangyo Co., Ltd. can be used, and pressurizing means such as a rubber ball or a syringe can be used in a simple place. Can also be used.
- the pressure in the pressurizing chamber 138 is set higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 130 during the reaction process, and more preferably maintained at 1 atm (1013 hPa) or more.
- the pressure in the pressurizing chamber 138 should be high enough to prevent significant sample evaporation and bubble generation that would affect the PCR reaction process even if the sample is repeatedly exposed to high temperatures (about 95 ° C.). Good.
- the higher the pressure in the pressurizing chamber 138 the more the influence of sample evaporation can be suppressed.
- the liquid feeding system 137 is complicated and enlarged including its handling, a person skilled in the art Can comprehensively judge the use, purpose, cost, and effect of the device and design the entire system.
- the pressure chamber 138 is provided with an atmospheric pressure release valve 148.
- the atmospheric pressure release valve 148 is controlled so that the pressure in the liquid feeding system 137 and the flow path 112 of the reaction processing container 110 becomes equal to the atmospheric pressure when the reaction processing container 110 is detached. As a result, it is possible to prevent the sample 120 from moving suddenly or jumping out.
- the pressure chamber 138 may be provided with a pressure sensor (not shown) for constantly monitoring the pressure in the internal space. By sending the actual pressure detected by the pressure sensor to the CPU 136, the pressure in the pressurizing chamber 138 can be suitably controlled.
- the reaction processing apparatus 130 further includes a fluorescence detector 150.
- the fluorescence from the sample 120 in the flow path 112 of the reaction processing container 110 can be detected using the fluorescence detector 150, and the value can be used as an index as a determination material for PCR progress or reaction termination.
- the optical fiber type fluorescence detector 150 includes a first optical head 151, a second optical head 154, a first fluorescence detector driver 152, a second fluorescence detector driver 155, a first optical head 151, and a first optical head.
- a first optical fiber 153 that connects the fluorescence detector driver 152 and a second optical fiber 156 that connects the second optical head 154 and the second fluorescence detector driver 155 are provided.
- the combination of the first optical head 151, the first fluorescence detector driver 152, and the first optical fiber 153 is referred to as a first fluorescence detector
- the second optical head 154, the second fluorescence detector driver 155, and the second optical fiber 156 are referred to as a first fluorescence detector.
- This combination can also be referred to as a second fluorescence detector.
- the first and second fluorescence detectors may have the same characteristics (for example, the same target wavelengths of excitation light and fluorescence), or may have different characteristics (for example, different target wavelengths). . In this case, it is advantageous in that it may be possible to know about amplification of a plurality of types of DNA having different fluorescence characteristics.
- the first optical head 151 is disposed in a flow path connecting the high temperature region 140 and the medium temperature region 141.
- the second optical head 154 is disposed in a flow path that connects the intermediate temperature region 141 and the low temperature region 142. Since the reaction of the sample 120 proceeds while being reciprocated in the flow path 112 and a predetermined DNA contained in the sample 120 is amplified, the progress of the amplification of the DNA is monitored by monitoring the variation in the amount of fluorescence obtained from the sample. Can be known in real time. In the continuous flow meandering flow path in one direction according to the first embodiment, it is substantially difficult to check the progress of DNA amplification in real time.
- reaction processing vessel comprising the reciprocating meandering flow path according to the second embodiment is also advantageous in this respect.
- a reaction processing method using the reaction processing apparatus 130 configured as described above will be described.
- the second end 146b of the first tube 146 is connected to the output of the first liquid pump 139, and the first end 146a of the first tube 146 is open.
- the second end 147b of the second tube 147 is connected to the output of the second liquid feeding pump 165, and the first end 147a of the second tube 147 is open.
- the reaction processing container 110 is placed on the reaction processing container mounting portion of the reaction processing apparatus 130.
- the atmospheric pressure release valve 148 provided in the pressurization chamber 138 is opened, and the first tube scheduled to be connected to the pressurization chamber 138 and the first communication port 117 and the second communication port 118 of the reaction processing vessel 110.
- the pressure in the second tube 147 is the same as the atmospheric pressure.
- the first end 146a of the first tube 146 extending from the first liquid feeding pump 139 is connected to the first communication port 117 of the reaction processing vessel 110, and the second tube 147 extending from the second liquid feeding pump 165 is used. Is connected to the second communication port 118 of the reaction processing vessel 110. None of the first liquid pump 139, the second liquid pump 165, and the pressurizing chamber pump 144 are operated at this time.
- the atmospheric pressure release valve 148 provided in the pressurizing chamber 138 is closed.
- the pressurizing chamber pump 144 is operated by the pressurizing chamber pump driver 145, and the pressure in the flow path 112 of the reaction processing vessel 110 communicating with the pressurizing chamber 138 and the pressure in the ambient environment of the reaction processing apparatus 130 is set. More preferably, the pressure is set to 1 atm (1013 hPa) or more.
- the pressure on the primary side and the secondary side are equal, that is, the first communication port 117 and the second side on the secondary side are the same.
- the pressure in the communication port 118 is also equal to the pressure in the pressurizing chamber 138.
- the sample 120 does not move.
- the pressure in the sample 120 and the flow path 112 including the sample 120 is always higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 130, and more preferably 1 atm or more. Therefore, even in a low atmospheric pressure environment such as a highland, the boiling point of the sample 120 made of an aqueous solution can be prevented from being lowered and the sample 120 can be prevented from boiling and foaming.
- the temperature control system 132 is operated to start temperature control of each temperature region in the reaction processing vessel 110. You may wait for predetermined time until the temperature of each temperature range becomes stable.
- the temperature control is preferably started after the pressure in the flow path 112 is maintained at a certain pressure or higher by the liquid feeding system 137.
- the initial position of the sample 120 is in the high temperature region 140, for example.
- the DNA is denatured.
- the first liquid feeding pump 139 is operated. Thereby, in the space on both sides of the sample 120, the pressure in the flow path 112 on the first communication port 117 side becomes higher than that on the second communication port 118 side, so that the sample 120 flows toward the second communication port 118.
- the inside of the path 112 can be pushed to move from the high temperature region 140 to the low temperature region 142 via the intermediate temperature region 141.
- the first liquid feeding pump 139 is stopped.
- the primary side pressure and the secondary side pressure of the liquid feed pump become equal as described above, so the space on the first communication port 117 side of the sample 120 and the second communication port 118.
- the pressure in the side channel space becomes equal to the pressure in the pressurizing chamber 138 (that is, there is no difference), and the movement of the sample 120 stops.
- DNA annealing is performed by placing the sample 120 in the low temperature region 142 for a certain period of time.
- the second liquid feeding pump 165 is operated, and when the movement of the sample 120 from the low temperature region 142 to the middle temperature region 141 is completed, the second liquid feeding pump 165 is stopped.
- the sample 120 is placed in the intermediate temperature region 141 for a certain period of time, thereby extending the DNA.
- the second liquid feeding pump 165 is operated to stop the second liquid feeding pump 165 when the movement of the sample 120 from the intermediate temperature region 141 to the high temperature region 140 is completed.
- the sample 120 is placed in the high temperature region 140 for a certain period of time to denature the DNA.
- the sample 120 reciprocates in the flow path 112. Specifically, samples of each temperature range of high temperature (denaturation)-low temperature (annealing)-medium temperature (elongation)-high temperature (denaturation)-low temperature (annealing)-medium temperature (elongation) ... 120 passes.
- the sample 120 passes through each temperature region in a cycle. Thereby, the sample 120 is given a predetermined number of thermal cycles, PCR occurs, and a predetermined DNA can be selectively amplified.
- the above-described fluorescence detector 150 can function as a position sensor. If the optical head of the fluorescence detector 150 is arranged to detect fluorescence emitted from the sample 120 at a specific location in the flow path 112, the fluorescence signal is zero when the sample 120 is not at that specific location. While at the background level, when the sample 120 passes through that particular location, the fluorescence signal rises from zero or the background level and shows an output variation that again becomes zero or the background level.
- a plurality of optical heads of the fluorescence detector 150 can be arranged along the flow path 112. For example, since the presence or absence of the sample 120 in each reaction region can be detected by arranging the optical head of the fluorescence detector 150 immediately below each reaction region, the sample 120 can be positioned more reliably.
- reaction processing method using the reaction processing apparatus 130 according to the second embodiment unlike the reaction processing method using the reaction processing apparatus 30 according to the first embodiment, during the reaction processing by the thermal cycle, it is advantageous in that the fluorescence from the sample 120 can be continuously detected and the progress of DNA amplification can be managed in real time as described above.
- the pressure in the flow path 112 of the reaction processing container 110 is always higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 130, preferably It is maintained at 1 atmosphere or more. That is, during the reaction process, the sample 120 is always pressurized to a pressure higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 130, preferably 1 atmosphere or more. Therefore, stable PCR can be performed while preventing boiling of the sample and generation of bubbles even in places with low atmospheric pressure such as in high altitudes or in airplanes.
- FIG. 8 is a schematic diagram for explaining a reaction processing apparatus 230 according to the third embodiment of the present invention.
- the same reaction processing container as the reaction processing container 110 (see FIG. 5) described in the second embodiment is used, the same components are denoted by the same reference numerals. A duplicate description will be omitted as appropriate.
- the same temperature control system 132 and fluorescence detector 150 as those described in the second embodiment are used for the temperature control system and the fluorescence detector in the reaction processing device 230, the same components are denoted by the same reference numerals. In addition, overlapping description will be omitted as appropriate.
- the reaction processing apparatus 230 according to the third embodiment of the present invention is different from the second embodiment in the configuration of the liquid feeding system and the reaction processing method based thereon.
- the liquid feeding system 237 of the reaction processing apparatus 230 controls the liquid feeding chamber 200, the pressurizing chamber 201, the liquid feeding chamber pump 202, and the liquid feeding chamber pump 202.
- Liquid pump pump 204 for pressurizing chamber, pressurizing chamber pump 203, pressurizing chamber pump driver 205 for controlling pressurizing chamber pump 203, first direction switching valve 206, and second A direction switching valve 207, a first tube 246, and a second tube 247 are provided.
- the reaction processing device 230 may include a driver (not shown) for controlling the first direction switching valve 206 and the second direction switching valve 207.
- FIG. 9 is a schematic diagram for explaining the configuration of the direction switching valve.
- the direction switching valve 900 shown in FIG. 9 can be used as the first direction switching valve 206 and the second direction switching valve 207 in the reaction processing apparatus 230 shown in FIG.
- the direction switching valve 900 includes a first supply port 901, a second supply port 902, and a discharge port 903.
- the direction switching valve 900 can switch communication between the first supply port 901 and the discharge port 903 and communication between the second supply port 902 and the discharge port 903.
- the communication switching means may be a direct-acting electromagnetic type or a pilot-type electromagnetic type that switches an internal valve by a separate air pressure.
- each path of the first supply port 901 and the discharge port 903 or the second supply port 902 and the discharge port 903 may be a so-called universal type valve in which air flows in both directions.
- a direction switching valve having four or more ports can also be used.
- the direction switching valve is not limited to these and may be a three-way cock.
- the first end 246 a of the first tube 246 is connected to the first communication port 117 of the reaction processing vessel 110. It is preferable that a packing or a seal for ensuring airtightness is disposed at a connection portion between the first communication port 117 and the first end portion 246a of the first tube 246.
- the second end 246 b of the first tube 246 is connected to the discharge port of the first direction switching valve 206. Further, the first supply port of the first direction switching valve 206 is connected to the liquid feeding chamber 200 by the hollow tube 210. Further, the second supply port of the first direction switching valve 206 is connected to the pressurizing chamber 201 by the hollow tube 211.
- the first end 247 a of the second tube 247 is connected to the second communication port 118 of the reaction processing vessel 110. It is preferable that a packing or a seal for ensuring airtightness is disposed at a connection portion between the second communication port 118 and the first end 247a of the second tube 247.
- the second end 247 b of the second tube 247 is connected to the discharge port of the second direction switching valve 207. Further, the first supply port of the second direction switching valve 207 is connected to the liquid feeding chamber 200 by the hollow tube 212. Further, the second supply port of the second direction switching valve 207 is connected to the pressurizing chamber 201 by the hollow tube 213.
- the liquid feeding chamber 200 forms a space having a constant volume therein.
- a liquid supply chamber pump 202 is connected to the liquid supply chamber 200.
- the liquid feeding chamber pump driver 204 controls the liquid feeding chamber pump 202 in accordance with an instruction from the CPU 236 so that the space in the liquid feeding chamber 200 becomes a predetermined pressure.
- the pressurizing chamber 201 forms a space having a constant volume therein.
- a pressurizing chamber pump 203 is connected to the pressurizing chamber 201.
- the pressurizing chamber pump driver 205 controls the pressurizing chamber pump 203 so that the space in the pressurizing chamber 201 becomes a predetermined pressure in accordance with an instruction from the CPU 236.
- liquid feeding chamber pump 202 and the pressurizing chamber pump 203 As the liquid feeding chamber pump 202 and the pressurizing chamber pump 203, a small DC diaphragm pump (model DSA-1-12BL) manufactured by Denso Sangyo Co., Ltd. can be used. A pressurizing means such as a syringe or the like can also be used.
- the pressure in the liquid feeding chamber 200 and the pressurizing chamber 201 is higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 130 during the reaction process, and more preferably maintained at 1 atm (1013 hPa) or more. Further, the pressure in the liquid feeding chamber 200 is maintained at a pressure higher than the pressure in the pressurizing chamber 201 during the reaction process.
- the liquid supply chamber 200 and the pressurization chamber 201 are provided with atmospheric pressure release valves 220 and 221, respectively.
- the atmospheric pressure release valves 220 and 221 can reset the pressure state inside the chamber when the reaction processing apparatus 230 is repeatedly used, and can prevent the sample 120 from abruptly moving or popping out when the reaction processing container 110 is detached. it can.
- a reaction processing method using the reaction processing apparatus 230 configured as described above will be described.
- the second end 246b of the first tube 246 is connected to the discharge port of the first direction switching valve 206, and the first end 246a of the first tube 246 is open.
- the second end 247b of the second tube 247 is connected to the discharge port of the second direction switching valve 207, and the first end 247a of the second tube 247 is open.
- the reaction processing container 110 is placed on the reaction processing container mounting portion of the reaction processing apparatus 230.
- the atmospheric pressure release valves 220 and 221 are opened, and the pressure in the liquid feeding chamber 200, the pressurizing chamber 201, the first direction switching valve 206, the second direction switching valve 207, the first tube 246, and the second tube 247 is adjusted. Same as atmospheric pressure. Subsequently, the first end 246a of the first tube 246 extending from the first direction switching valve 206 is connected to the first communication port 117 of the reaction processing vessel 110, and the second tube 247 extending from the second direction switching valve 207 is connected to the first end 246a. One end 247 a is connected to the second communication port 118 of the reaction processing vessel 110. Neither the liquid feeding chamber pump 202 nor the pressurizing chamber pump 203 is operated at this time. Subsequently, the atmospheric pressure release valves 220 and 221 are closed.
- the first direction switching valve 206 and the second direction switching valve 207 are operated to switch to a path in which the second supply port communicating with the pressurizing chamber 201 and the discharge port communicate with each other.
- the pump 203 is operated.
- the pressurizing chamber 201 is higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 130, more preferably increased to 1 atm (1013 hPa) or more.
- the pressurizing chamber 201 communicates with the first communication port 117 and the second communication port 118 of the reaction processing vessel 110 through the second supply port and the discharge port of the first direction switching valve 206 and the second direction switching valve 207. Yes. Accordingly, the pressure on both sides of the sample 120 (the first communication port 117 side and the second communication port 118 side) becomes equal even when the pressure in the pressurizing chamber 201 is increased. Do not move.
- the temperature control system 132 is operated to start temperature control in each temperature region in the reaction processing vessel 110. You may wait for predetermined time until the temperature of each temperature range becomes stable.
- the liquid feeding chamber pump 202 is operated to raise the pressure in the liquid feeding chamber 200.
- the liquid feeding chamber 200 is not in communication with the space (the first communication port 117 side and the second communication port 118 side) on both sides of the sample 120 in the flow path of the reaction processing container 110.
- the pressure in the channel does not affect the pressure in the flow path, and the sample 120 does not move.
- the pressure in the liquid feeding chamber 200 is higher than the pressure in the pressurizing chamber 201. This difference in pressure becomes a driving force for moving the sample 120.
- the initial position of the sample 120 is, for example, in the high temperature region 140 shown in FIG.
- the DNA is denatured.
- the first direction switching valve 206 is operated to switch to a path in which the first supply port and the discharge port communicate with each other.
- the space on the first communication port 117 side of the sample 120 becomes equal to the pressure in the liquid feeding chamber 200, and the pressure in the space on the first communication port 117 side becomes higher than the pressure on the second communication port 118 side.
- the sample 120 is pushed through the flow path 112 toward the second communication port 118 and can move from the high temperature region 140 to the low temperature region 142 via the intermediate temperature region 141.
- the first direction switching valve 206 When the sample 120 reaches the low temperature region 142, the first direction switching valve 206 is operated to switch to a path in which the second supply port and the discharge port communicate with each other. Thereby, the space on the first communication port 117 side of the sample 120 is also the same as the pressure in the pressurizing chamber 201, and the pressure in the space on the first communication port 117 side is equal to the pressure on the second communication port 118 side. Therefore, the movement of the sample 120 stops.
- DNA annealing is performed by placing the sample 120 in the low temperature region 142 for a certain period of time.
- the second direction switching valve 207 is operated to switch to a path in which the first supply port and the discharge port communicate with each other.
- the space on the second communication port 118 side of the sample 120 becomes the same as the pressure in the liquid feeding chamber 200, and the pressure in the space on the second communication port 118 side becomes higher than the pressure on the first communication port 117 side.
- the sample 120 is moved in the flow path toward the first communication port 117 and can move from the low temperature region 142 to the intermediate temperature region 141.
- the second direction switching valve 207 is operated to switch to a path in which the second supply port and the discharge port communicate with each other.
- the space on the second communication port 118 side of the sample 120 is also the same as the pressure in the pressurizing chamber 201, and the pressure on the second communication port 118 side and the pressure on the first communication port 117 side are equal.
- the movement of the sample 120 stops.
- DNA is extended by placing the sample in the intermediate temperature region 141 for a certain period of time.
- the second direction switching valve 207 is operated to switch to a path in which the first supply port and the discharge port communicate with each other.
- the sample 120 is pushed in the flow path 112 toward the first communication port 117 and can move from the intermediate temperature region 141 to the high temperature region 140.
- the second direction switching valve 207 is operated to switch to a path in which the second supply port and the discharge port communicate with each other.
- the space on the second communication port 118 side of the sample 120 is also the same as the pressure in the pressurizing chamber 201, and the pressure on the second communication port 118 side is equal to the pressure on the first communication port 117 side. Therefore, the movement of the sample 120 stops.
- DNA is denatured by placing the sample in the high temperature region 140 for a certain period of time.
- the sample 120 reciprocates in the flow path 112. be able to. Specifically, samples of each temperature range of high temperature (denaturation)-low temperature (annealing)-medium temperature (elongation)-high temperature (denaturation)-low temperature (annealing)-medium temperature (elongation) ... 120 passes.
- the sample 120 passes through each temperature region in a cycle. Thereby, the sample 120 is given a predetermined number of thermal cycles, PCR occurs, and a predetermined DNA can be selectively amplified.
- the pressure in the flow path 112 of the reaction processing container 110 is always higher than the atmospheric pressure in the surrounding environment of the reaction processing apparatus 230, more preferably. Is maintained above 1 atm. That is, the sample 120 is always higher than the ambient pressure maintained in the pressurization chamber 201, more preferably 1 atm (1013 hPa) or higher, or higher than the pressure in the pressurization chamber 201. Pressurization is performed by the pressure in the liquid chamber 200. Therefore, PCR can be performed while preventing boiling of the sample and generation of bubbles even in places with low atmospheric pressure such as in high altitudes or in airplanes.
- reaction processing apparatus has been described above.
- a reaction processing apparatus that does not depend on the reaction processing apparatus according to the present invention, that is, in the case of a reaction processing apparatus that does not pressurize a sample in a flow path, when PCR is performed in a high altitude or a low atmospheric pressure environment in an aircraft
- the sample may boil easily and foam. Foamed foam often occurs in the middle of the sample, and more often it occurs. If this happens, the pressure inside the bubble generated between the sample and the pressure for liquid delivery, etc. will start to balance, and a part of the sample may stop in the flow path, causing a phenomenon that the liquid delivery cannot be performed smoothly. .
- the reaction processing apparatus of the present invention since the probability of foaming can be dramatically reduced in the first place, the above-mentioned problems do not occur, and the sample is fed under any atmospheric pressure environment. As a result, an amplified sample such as DNA can be obtained by a stable reaction treatment.
- the present invention can be used for polymerase chain reaction (PCR).
- PCR polymerase chain reaction
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Abstract
Description
図1(a)および(b)は、本発明の第1実施形態に係る反応処理装置で使用可能な反応処理容器10を説明するための図である。図1(a)は、反応処理容器10の平面図であり、図1(b)は、反応処理容器10の正面図である。
図5(a)および(b)は、本発明の第2実施形態に係る反応処理装置で使用可能な反応処理容器110を説明するための図である。図5(a)は、反応処理容器110の平面図であり、図5(b)は、反応処理容器110の正面図である。
図8は、本発明の第3実施形態に係る反応処理装置230を説明するための模式図である。本第3実施形態に係る反応処理装置230では、反応処理容器は第2実施形態で説明した反応処理容器110(図5参照)と同じものを使用するので、同一の構成要素には同じ符号を付し、重複する説明を適宜省略する。また、反応処理装置230における温度制御システムおよび蛍光検出器についても第2実施形態で説明した温度制御システム132および蛍光検出器150と同じものを使用するため、同一の構成要素には同じ符号を付し、重複する説明を適宜省略する。本発明の第3実施形態に係る反応処理装置230は、送液システムの構成と、それに基づく反応処理方法が第2実施形態と異なる。
Claims (14)
- 試料が流路内を移動して、該試料にサーマルサイクルを与えることによって、試料の反応処理を行う反応処理装置において、
反応処理中の前記流路内の圧力を、前記反応処理装置の周辺環境の気圧より高く維持することを特徴とする反応処理装置。 - 前記流路内の気圧は1気圧以上であることを特徴とする請求項1に記載の反応処理装置。
- 前記流路内の試料の両側に生じた圧力の差を、試料が前記流路内を移動するための推進力とすることを特徴とする請求項1又は2に記載の反応処理装置。
- 前記流路内の試料の両側に生じた圧力を、略等しくすることによって、試料が前記流路内で停止することを特徴とする請求項1から3のいずれかに記載の反応処理装置。
- 試料が反応処理容器の流路内を移動して、該試料にサーマルサイクルを与えることによって、試料の反応処理を行う反応処理装置において、
前記試料を前記流路内で移動及び停止させるために、前記反応処理容器の前記流路内の圧力を制御する送液システムを備え、
前記送液システムは、前記試料の反応処理中に、前記流路内の圧力を、前記反応処理装置の周辺環境の気圧より高く維持することを特徴とする反応処理装置。 - 前記送液システムは、
内部の圧力が前記反応処理装置の周辺環境の気圧より高く維持された加圧チャンバと、
前記加圧チャンバ内に配置された送液用ポンプと、
を備え、
前記送液用ポンプの出力と、前記反応処理容器の流路の一端に設けられた第1連通口とが連通され、
前記加圧チャンバの内部と、前記反応処理容器の流路の他端に設けられた第2連通口とが連通され、
前記試料を前記流路内で移動させるために、前記送液用ポンプを制御する制御部をさらに備えることを特徴とする請求項5に記載の反応処理装置。 - 前記送液システムは、
内部の圧力が前記反応処理装置の周辺環境の気圧より高く維持された加圧チャンバと、
前記加圧チャンバ内に配置された第1送液用ポンプと、
前記加圧チャンバ内に配置された第2送液用ポンプと、
を備え、
前記第1送液用ポンプの出力と、前記反応処理容器の流路の一端に設けられた第1連通口とが連通され、
前記第2送液用ポンプの出力と、前記反応処理容器の流路の他端に設けられた第2連通口とが連通され、
前記試料を前記流路内で移動させるために、前記第1送液用ポンプおよび前記第2送液用ポンプを制御する制御部をさらに備えることを特徴とする請求項5に記載の反応処理装置。 - 前記送液用ポンプは停止時には、一次側と二次側の圧力が等しくなることを特徴とする請求項6又は7に記載の反応処理装置。
- 前記送液システムは、
内部の圧力が前記反応処理装置の周辺環境の気圧より高く維持された加圧チャンバと、
内部の圧力が前記加圧チャンバ内よりも高い圧力に維持された送液チャンバと、
前記加圧チャンバと前記送液チャンバのいずれか一方を前記反応処理容器の流路の一端に設けられた第1連通口に連通させる第1方向切換バルブと、
前記加圧チャンバと前記送液チャンバのいずれか一方を前記反応処理容器の流路の他端に設けられた第2連通口に連通させる第2方向切換バルブと、
を備え、
前記試料を前記流路内で移動させるために、第1方向切換バルブおよび第2方向切換バルブを制御する制御部をさらに備えることを特徴とする請求項5に記載の反応処理装置。 - 前記試料は、DNAと、PCR試薬と、蛍光を発する試薬を含み、
前記反応処理はPCRであることを特徴とする請求項1から9のいずれかに記載の反応処理装置。 - 前記反応処理装置は、前記流路中の試料から発せられる蛍光を検出するための、一又は二以上の蛍光検出器を備え、該蛍光検出器からの信号に基づいて試料を移動させることを特徴とする請求項10に記載の反応処理装置。
- それぞれ異なる温度に維持された複数の温度領域と、それらの温度領域を接続する流路と、からなるサーマルサイクル領域を備え、
前記蛍光検出器は、前記温度領域を接続する流路中の試料からの蛍光を検出するように配置されていることを特徴とする請求項11に記載の反応処理装置。 - 反応処理装置に適用される反応処理容器であって、
試料が前記反応処理装置の流路内を移動して、該試料にサーマルサイクルを与えることによって、試料の反応処理を行い、
反応処理中の前記流路内の圧力を、前記反応処理装置の周辺の気圧より高く維持することを特徴とする反応処理容器。 - 試料が導入される流路を備える反応処理容器を載置する工程と、
前記流路内の試料を加熱するために、前記流路の温度を制御する工程と、
前記試料を前記流路内で移動するために、前記反応処理容器の前記流路内の圧力を制御する工程と、
を備え、
前記試料の反応処理中に、前記流路内の圧力が前記反応処理容器の周辺の気圧より高く維持されることを特徴とする反応処理方法。
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JP2021027830A (ja) | 2021-02-25 |
JP7223736B2 (ja) | 2023-02-16 |
EP3401386A1 (en) | 2018-11-14 |
CN108431199A (zh) | 2018-08-21 |
US20180311673A1 (en) | 2018-11-01 |
SG10201911933TA (en) | 2020-02-27 |
CN108431199B (zh) | 2022-04-08 |
SG11201805707VA (en) | 2018-07-30 |
US11351552B2 (en) | 2022-06-07 |
EP3401386A4 (en) | 2019-12-25 |
JPWO2017119382A1 (ja) | 2018-11-08 |
JP6792845B2 (ja) | 2020-12-02 |
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