WO2005054844A1 - 反応容器およびそれを利用する反応装置および検出装置および反応容器の作製方法 - Google Patents
反応容器およびそれを利用する反応装置および検出装置および反応容器の作製方法 Download PDFInfo
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- WO2005054844A1 WO2005054844A1 PCT/JP2004/018063 JP2004018063W WO2005054844A1 WO 2005054844 A1 WO2005054844 A1 WO 2005054844A1 JP 2004018063 W JP2004018063 W JP 2004018063W WO 2005054844 A1 WO2005054844 A1 WO 2005054844A1
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- reaction vessel
- solution
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- B01L3/50—Containers for the purpose of retaining a material to be analysed, e.g. test tubes
- B01L3/508—Containers for the purpose of retaining a material to be analysed, e.g. test tubes rigid containers not provided for above
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- B01J2219/00378—Piezoelectric or ink jet dispensers
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- B01J2219/00583—Features relative to the processes being carried out
- B01J2219/00603—Making arrays on substantially continuous surfaces
- B01J2219/00639—Making arrays on substantially continuous surfaces the compounds being trapped in or bound to a porous medium
- B01J2219/00641—Making arrays on substantially continuous surfaces the compounds being trapped in or bound to a porous medium the porous medium being continuous, e.g. porous oxide substrates
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Definitions
- reaction vessel Reaction vessel, reaction apparatus and detection apparatus using the same, and method of manufacturing reaction vessel
- the present invention relates to a reaction container used for detecting a biological substance, a reaction device using this reaction container, and a detection device.
- WO 03Z027673 the present applicant has proposed a gene testing apparatus using a three-dimensional DNA microarray, which can easily and quickly test a gene.
- the reaction solution is put into a reaction container of a three-dimensional DNA microarray using a porous filter as a carrier, and repeatedly passed through the reaction part by, for example, pressurization and decompression by a syringe pump.
- a genetic test can be performed with good reproducibility in a short time.
- WO 03Z005013 proposes a microarray having a structure in which a porous substrate is used and a reaction solution is repeatedly passed through a reaction section by a syringe or a piston. Disclosure of the invention
- reaction solution is dispensed into the reaction vessel by the upward force of the microarray substrate, and the reaction state is measured from the top. Observation is performed, and the pressure is reduced and increased by the syringe pump from below. For this reason, manual dispensing is required, and when handling a large number of samples, much time is required.
- a secondary object of the present invention is to provide a novel reaction vessel for providing a technique relating to such a biological substance.
- Another secondary object of the present invention is to provide a reactor utilizing such a reaction vessel.
- Another object of the present invention is to provide a novel detection device using such a reaction vessel.
- the present invention is directed, in part, to a reaction container for detecting a biological substance.
- the reaction container of the present invention comprises a three-dimensional base material on which a probe for detecting a biological substance is immobilized, and a connecting portion which can be airtightly connected to the liquid driving means and can be connected to the detecting means so as not to leak light. And a solution suction part capable of sucking the solution.
- the connection part and the solution suction part are connected with a three-dimensional base material interposed therebetween.
- the present invention is directed, in part, to an apparatus for reacting a biological substance using the above-described reaction container.
- the reaction apparatus according to the present invention includes: a fitting portion that can be fitted to the coupling portion of the reaction vessel; pressure control means for transmitting pressure for sucking and discharging the sample solution to the reaction vessel through the fitting portion; And a temperature adjusting means for adjusting the temperature of the sample solution inside.
- the present invention is directed, in part, to an apparatus for detecting a biological substance using the above-described reaction container.
- the detection device of the present invention has a fitting portion that can be fitted to a coupling portion of a reaction container, and a detection unit that detects a reaction of a biological substance on a three-dimensional base material in the reaction container.
- FIG. 1 schematically shows a reaction vessel and an inspection device according to a first embodiment of the present invention.
- FIG. 2 is a sectional view of an inspection device and a reaction vessel according to a second embodiment of the present invention.
- FIG. 3 schematically shows a configuration of an observation optical system and a reaction vessel according to a second embodiment of the present invention.
- FIG. 4 is a perspective view schematically showing a configuration of an inspection device according to a fourth embodiment of the present invention.
- FIG. 5 shows the temperature control unit shown in FIG. 4 and a temperature controller connected thereto.
- FIG. 6 schematically shows a reaction container and an inspection device according to a fifth embodiment of the present invention.
- FIG. 7 is a cross-sectional view of an inspection device and a reaction vessel according to a sixth embodiment of the present invention.
- FIG. 8 shows a pressure change in the inspection device shown in FIG. 7.
- FIG. 9 is a sectional view of a reaction vessel according to a seventh embodiment of the present invention.
- FIG. 10 schematically illustrates a configuration of an inspection device according to an eighth embodiment of the present invention.
- FIG. 11 is a perspective view of an inspection device according to a tenth embodiment of the present invention.
- FIG. 12 shows the reaction vessel transport guide shown in FIG. 11, and shows a state in which the reaction vessel is housed inside the reaction vessel transport guide.
- FIG. 13 shows the reaction container transport guide shown in FIG. 11, and shows a state in which the reaction container is lowered and protrudes from the reaction container transport guide.
- FIG. 14 schematically shows a configuration of an inspection device according to an eleventh embodiment of the present invention.
- FIG. 15 is a plan view of the fitting section shown in FIG. 14 as viewed from below.
- FIG. 16 schematically shows a configuration of an inspection apparatus according to a twelfth embodiment of the present invention.
- FIG. 17 schematically shows a configuration of an inspection device according to a thirteenth embodiment of the present invention.
- FIG. 18 schematically shows a configuration of an inspection apparatus according to a fourteenth embodiment of the present invention.
- FIG. 19 is a plan view schematically showing a configuration of an inspection device according to a fifteenth embodiment of the present invention.
- FIG. 20 schematically shows a cross section of the turntable shown in FIG.
- FIG. 21 schematically shows the sample collecting apparatus shown in FIG.
- FIG. 22 schematically shows a cross section of a peripheral portion of the reaction vessel supply device shown in FIG.
- FIG. 23 shows the first step in the method for producing a reaction vessel according to the sixteenth embodiment of the present invention.
- FIG. 24 shows the next step following the step shown in FIG. 23.
- FIG. 25 shows the next step following the step shown in FIG. 24.
- FIG. 26 shows the next step following the step shown in FIG. 25.
- FIG. 27 shows the next step following the step shown in FIG. 26.
- FIG. 28 shows the next step that follows the step shown in FIG. 27.
- FIG. 29 shows the first step in the method for producing a reaction vessel according to the seventeenth embodiment of the present invention.
- FIG. 30 shows a next step following the step shown in FIG. 29.
- FIG. 31 shows a next step following the step shown in FIG. 30.
- FIG. 32 shows the first step in the method for producing a reaction vessel according to the eighteenth embodiment of the present invention.
- FIG. 33 shows the next step following the step shown in FIG. 32.
- FIG. 34 shows the next step following the step shown in FIG. 33.
- FIG. 35 shows the first step in the method for producing a reaction vessel according to the eighteenth embodiment of the present invention.
- FIG. 36 shows a sectional structure of a three-dimensional substrate formed by the process shown in FIG. 35.
- FIG. 37 shows the next step following the step shown in FIG. 35.
- FIG. 38 shows the next step following the step shown in FIG. 37.
- FIG. 39 shows the next step following the step shown in FIG.
- FIG. 40 shows the next step following the step shown in FIG. 39.
- the present embodiment is directed to a novel reaction container for detecting a biologically related substance and a biologically related substance inspection apparatus (reactor and detector) using the same.
- bio-related substance includes not only cells of animals, plants, microorganisms, and the like, but also substances derived from viruses and the like that cannot proliferate without parasitism. No. Bio-related substances are extracted directly from these cells, etc. In addition, it includes those produced using genetic engineering techniques and those chemically modified. More specifically, they include hormones, enzymes, antibodies, antigens, abzymes, other proteins, nucleic acids, and the like.
- probe refers to a substance that specifically binds to the above-mentioned biologically relevant substance.
- a ligand such as a hormone and its receptor, an enzyme and its substrate, an antigen and its antigen, and the like.
- Body a nucleic acid having a specific sequence and a nucleic acid having a sequence complementary thereto, and the like.
- FIG. 1 schematically shows a reaction vessel and an inspection device according to a first embodiment of the present invention.
- a reaction vessel 101 includes a three-dimensional substrate 102 on which a probe for detecting a biological substance is immobilized, a coupling part 103 coupled to an inspection device, and a solution. And a solution inhalation part 104 capable of inhalation.
- a "three-dimensional substrate” refers to a substrate on which a probe is immobilized, has a structure that has a three-dimensional spread and can substantially pass a liquid.
- Any material and structure can be used.
- various filters and porous materials can be used.
- porous bodies, hollow fibers, metal oxide films, beads, and cavities obtained by etching a Si wafer are preferable.
- the three-dimensional substrate 102 includes a reaction region in which a plurality of probe molecules for capturing a target substance are immobilized in a circular shape having a diameter of 120 m.
- the connection part 103 and the solution suction part 104 are connected with the three-dimensional substrate 102 interposed therebetween.
- the coupling part 103 and the solution suction part 104 are made of a non-light-transmitting material.
- the inspection device moves the fitting portion 111 that can be fitted to the coupling portion 103 of the reaction vessel 101, the pressure control section 112 that controls the pressure of the reaction vessel 101 through the fitting portion 111, and the fitting portion 111. And a biaxial robot 113 that supports the robot.
- the pressure control section 112 has a means for generating pressure and a means for detecting pressure.
- the inspection device also has a sample container 114 for storing a sample solution and a cleaning liquid container 115 for storing a cleaning liquid.
- the sample container 114 is made of, for example, a microtiter plate.
- the washing liquid container 115 is constituted by, for example, a microtiter plate or a bottle.
- the coupling portion 103 of the reaction vessel 101 has an open end, and the fitting portion 111 is fitted to the opening end of the coupling portion 103, so that the reaction vessel 101 can be detached from the fitting portion 111. It is attached to.
- the reaction vessel 101 attached to the fitting section 111 is airtightly connected to the pressure control section 112.
- the two-axis robot 113 can move the reaction vessel 101 attached to the fitting part 111.
- the pressure control unit 112 transmits a pressure to the reaction container 101 attached to the fitting unit 111, so that the sample solution or the cleaning liquid is supplied from the sample container 114 or the cleaning liquid container 115 through the solution suction unit 104. Inhalation into 101 and draining of sample solution and washing solution in reaction vessel 101.
- the inspection apparatus further includes a heater 116 for controlling the sample temperature during the hybridization reaction and the cleaning solution temperature during the cleaning, a temperature measuring resistor 117 for measuring the temperature of the heater 116, and a thermometer. It has a temperature control section 118 for controlling the temperature of the heater 116 based on the information obtained by the resistor 117.
- the heater 116 has a space for accommodating the reaction vessel 101.
- the reaction vessel 101 attached to the fitting portion 111 is moved into this space of the heater 116 by the two-axis robot 113 as necessary.
- the heater 116, the resistance temperature detector 117, and the temperature control unit 118 constitute a temperature adjusting means for adjusting the temperature of the solution in the reaction vessel 101.
- the temperature adjusting means cooperates with the fitting section 111 and the pressure control section 112 to constitute a reaction device for promoting the hybridization reaction.
- the inspection apparatus further has an observation optical system 120 for optically observing the three-dimensional substrate 102 in the reaction vessel 101.
- the observation optical system 120 is, for example, a fluorescence observation optical system.
- the observation optical system 120 includes a light source 122 that emits light having a visible wavelength, an optical power generated by the light source 122, an excitation filter 123 that selectively transmits a wavelength for exciting a fluorescent substance bound to a sample molecule, and an excitation filter.
- a dichroic mirror 124 that reflects light transmitted through 123 and selectively transmits fluorescence generated from a fluorescent substance, and a fluorescent filter 125 that selectively transmits fluorescent light generated from a fluorescent substance and transmitted through dichroic mirror 124.
- the observation optical system 120 further includes a sample molecule to a probe molecule on the three-dimensional substrate 102.
- An objective lens 126 for optically detecting the capture of light, an illumination optical system 127 for guiding light from a light source 122 to a three-dimensional substrate 102 through an excitation filter 123 and a dichroic mirror 124, and an objective lens 126.
- An imaging optical system 128 for imaging light from the three-dimensional substrate 102, and a CCD camera 129 for converting an optical image formed by the imaging optical system 128 into an electric signal! / Puru.
- the coupling portion 103 has a tapered inner surface whose diameter increases as the distance from the three-dimensional substrate 102 increases.
- the coupling section 103 has an open end into which the fitting section 111 is inserted, and the taper angle between the open end and the three-dimensional base 102 is larger than the NA of the objective lens 126.
- a fluorescent substance such as FITC
- the dissolved sample solution is dispensed into the sample container 114 and set at the sample container setting position.
- the washing liquid is dispensed into the washing liquid container 115 and set at the washing liquid container setting position.
- the reaction vessel 101 is set at a predetermined position.
- the reaction vessel 101 is mounted on the fitting part 111.
- the pressure inside the reaction vessel 101 is reduced by the pressure control section 112 through the fitting section 111, and the sample solution is sucked from the sample vessel 114.
- the solution suction portion 104 of the reaction vessel may have residual force such as a microtiter plate, especially when aspirating the sample solution. It is preferable because the amount is reduced.
- the air layer is suctioned after suctioning the sample solution, the sample solution does not hang down on the reaction container when moving to the temperature control unit.Furthermore, when the sample solution is moved up and down the three-dimensional substrate, The sample solution does not drip in the reaction vessel preferable.
- the reaction vessel 101 is attached to the recess of the heater 116 so as to be in close contact therewith.
- the heater 116 is controlled to a desired temperature.
- the pressure control unit 112 repeatedly pressurizes and depressurizes the inside of the reaction vessel 101 to move the sample solution above and below the three-dimensional substrate 102 to hybridize the probe and the nucleic acid contained in the sample solution. Let it.
- the pressure control unit 112 pressurizes the inside of the reaction container 101 via the fitting unit 111, and the sample solution is discarded in the sample container 114.
- the pressure inside the reaction vessel 101 is reduced by the pressure control section 112 through the fitting section 111, and the cleaning liquid is sucked from the cleaning liquid container 115.
- the pressure control unit 112 repeatedly pressurizes and depressurizes the inside of the reaction vessel 101 to wash the three-dimensional base material 102 with a washing solution, which is included in a small sample solution that does not bind to probe molecules. Wash out the nucleic acid!
- the three-dimensional substrate 102 is exposed by removing the reaction container 101 from the fitting part 111.
- the observation optical system 120 is arranged above the reaction vessel 101. By irradiating the excitation light, light from the probe spot on the three-dimensional substrate 102 is photographed as electronic image data by the CCD camera 129, and the image and data on the light amount of the probe spot are stored.
- the stored data is analyzed to examine the expression state, mutation, polymorphism, etc. of the nucleic acid contained in the sample solution.
- one pressure control unit 112 can aspirate a solution required for testing a biologically related substance such as a sample solution and a washing solution from each container, and can use the sample solution and the washing solution together with the sample solution. Move the sample solution to make the porous body contact efficiently. Can be made. In other words, the dispensing mechanism for the sample solution and the washing solution and the driving mechanism for the sample solution are shared. For this reason, the device configuration is simplified.
- a solution required for testing a biologically relevant substance such as a sample solution or a washing solution be placed in a microtiter plate.
- the sample container 114 and the washing solution container 115 are constituted by microtiter plates. In that case, it is possible to inspect a large number of samples at high speed.
- the reaction vessel 101 does not substantially transmit light, it is preferable to perform an inspection using light such as fluorescence or chemiluminescence because it is not necessary to provide special light shielding means.
- light such as fluorescence or chemiluminescence
- the reaction vessel 101 has a light shielding function.
- the material is not particularly limited as long as it can substantially shield light, but a crystalline resin is preferable from the viewpoint of chemical resistance to the solution to be handled and heat resistance. Examples of the crystalline resin include polypropylene, polyacetal, polyamide-based synthetic resin, polymethylpentene, polyethylene terephthalate, and polyethylene.
- polypropylene and polyacetal containing carbon particles are more preferable because they can impart a sufficient light-shielding function.
- polyacetal is particularly preferable because it can produce a reaction container having high transferability from a molding die and high dimensional accuracy.
- the inner surface of the joint 103 of the reaction vessel 101 has a taper, and the taper angular force between the open end of the joint 103 and the three-dimensional substrate 102 is larger than the NA of the objective lens 126.
- the NA of the observation optical system 120 In order to efficiently receive all signals from a spot without the optical system becoming too large, the NA of the observation optical system 120 must be substantially equal to the taper angle of the inner surface of the coupling portion 103 of the reaction vessel 101. Particularly preferred.
- the reaction vessel 101 having such a taper can be mass-produced by molding using resin, and it is sufficient that the resin has a thickness of about 0.1 to 0.2 mm or less. Since a container having strength can be manufactured, the heat capacity is reduced, and the temperature response is increased, so that a biologically relevant substance can be accurately inspected.
- the diameter of the portion of the reaction vessel 101 where the three-dimensional base material 102 is arranged is preferably 11 to 16 mm. In clinical tests, the number of spots is considered to be about 10-250 based on the number of test items. For example, when testing about 30 single nucleotide polymorphisms, 240 types of probes are required because 8 types of probes may be required for each single nucleotide polymorphism. Therefore, when this probe is immobilized on a three-dimensional substrate, if the diameter of the inspection container at the part where the three-dimensional substrate is to be placed is 16 mm, spots of about 10 to 250 are efficiently arranged. I like it because it becomes possible.
- a biological substance as a test substance is extracted by sampling blood and tissue strength. Therefore, the amount that can be sampled is limited. It is desirable that the test can be performed with as small a volume as possible.However, if the volume of the sample solution is small, the reaction temperature in the reaction stage is often set to a predetermined temperature of about 30 ° C to 60 ° C. May affect test results. Furthermore, in order to carry out the reaction and detection of biological substances with good reproducibility, a certain volume is necessary, considering the movement of the solution, the maintenance of the temperature, and the evaporation of the solution, and it is 10 to 100 L. Thus, the reaction and detection of a biological substance can be performed with good reproducibility.
- the volume of the sample solution finally adjusted is 10-100 / zL.
- the actual volume of the reaction vessel 101 is 10-100 / zL. It is preferred that there is.
- the reaction and detection can be performed in a very short time. No. Inspection can be performed at high throughput.
- FIG. 2 is a sectional view of an inspection device and a reaction vessel according to a second embodiment of the present invention.
- members indicated by the same reference numerals as the members shown in FIG. 1 are the same members, and a detailed description thereof will be omitted.
- the fitting portion 130 in the present embodiment includes an observation optical system for optically observing the three-dimensional base material 102. That is, the fitting portion 130 includes an imaging optical system 131 for forming an optical image of the three-dimensional base material 102, and the three-dimensional base material 102 formed by the imaging optical system 131. It has a CCD 132 for converting the optical image into an electric signal, and an LED 133 for emitting light having a wavelength capable of exciting fluorescent molecules bonded to the sample molecules.
- the fitting section 130 is connected to the pressure control section 112 (see FIG. 1), like the fitting section 111 of the first embodiment. Therefore, the inside of the reaction vessel 101 can be pressurized or depressurized by the pressure control unit 112.
- the observation optical system is provided in the fitting part 130, the three-dimensional base material in the reaction vessel 101 can be removed without removing the reaction vessel 101 from the fitting part 130. 102 can be observed optically.
- the fitting unit 130 can transmit the pressure from the pressure control unit 112 to the reaction vessel 101, similarly to the fitting unit 111 of the first embodiment, the reaction can be performed while driving the sample solution. It is also possible to observe a change in state. In order to perform the measurement under the optimal condition for each probe, perform the measurement under one condition and then perform the measurement under another condition. For example, if one probe measures at 40 ° C and another probe measures at 60 ° C, or when measuring while changing the temperature or changing the reaction conditions, Particularly preferred. It is also possible to determine the appropriate reaction time by measuring the change over time.
- FIG. 3 schematically shows a configuration of an observation optical system and a reaction vessel according to a second embodiment of the present invention.
- members indicated by the same reference numerals as the members shown in FIG. 1 are the same members, and detailed description thereof will be omitted.
- the observation optical system 120A of the present embodiment includes optical elements functionally similar to the optical elements of the observation optical system 120 of the first embodiment. Further, the observation optical system 120A has a sleeve 160 that can be fitted to the coupling portion 103 of the reaction vessel 101. The sleeve 160 is also constructed of a non-light transmitting material. The objective lens 126 is accommodated and held in the sleeve 160.
- observation optical system 120A are functionally the same as the optical elements of the observation optical system 120 of the first embodiment, but their size is the same as that of the observation light of the first embodiment. Very small compared to 120 optical elements.
- observation of the three-dimensional substrate 102 in the reaction vessel 101 is performed in a state where the sleeve 160 containing the objective lens 126 is fitted to the coupling portion 103 of the reaction vessel 101.
- the sleeve 160 accommodating the objective lens 126 is fitted into the coupling portion 103 of the reaction vessel 101, the space between the three-dimensional base material 102 and the objective lens 126 can be made good optically. Is shut off. For this reason, the incidence of disturbance light on the observation optical system 120A is favorably prevented. Therefore, measurement accuracy is improved.
- FIG. 4 is a perspective view schematically showing a configuration of an inspection device according to a fourth embodiment of the present invention.
- FIG. 5 shows the temperature control unit shown in FIG. 4 and a temperature controller connected thereto. 4 and 5, the members indicated by the same reference numerals as those shown in FIG. 1 are the same members, and the detailed description thereof will be omitted.
- the inspection apparatus of the present embodiment positions the rack 141 for storing the reaction vessel 101, the microplate 142 for storing the sample solution or the washing solution, and the rack 141.
- a base 145 having a rack housing 143 on which a microplate 142 can be mounted and a rack housing 143 on which a microplate 142 can be mounted, and a fitting portion 111 which can be fitted into the reaction vessel 101 as in the first embodiment. It has an XYZ robot 146 that movably supports the fitting portion 111, and a temperature adjustment unit 147 for adjusting the temperature of the solution in the reaction vessel 101.
- the rack 141 only needs to be able to accommodate at least the reaction vessels 101, and more preferably, it is desirable to be able to accommodate a plurality of reaction vessels 101.
- the fitting portion 111 is connected to the pressure control unit 112 (see FIG. 1), like the fitting portion 111 of the first embodiment.
- FIG. 4 shows the inspection apparatus as having only one fitting portion 111, it is more preferable that the inspection apparatus be operated so that a plurality of reaction vessels 101 can be operated at the same time.
- the device has a plurality of fitting portions 111! /
- the temperature control unit 147 has a concave portion 150 that can accommodate the reaction vessel 101 in substantially contact therewith.
- the recess 150 does not hinder the movement of the solution in the reaction vessel 101. It is connected to the outside through a hole at the lower end.
- the temperature control unit 147 has a Peltier element 148 for temperature control and a thermocouple 149 for temperature detection. Both the Peltier element 148 and the thermocouple 149 are electrically connected to a temperature controller 151 that controls the temperature of the temperature control unit 147.
- the temperature controller 151 controls driving of the Peltier element 148 based on information obtained by the thermocouple 149.
- the inspection apparatus of the present embodiment has an observation optical system 120A similar to that of the third embodiment, and an XYZ robot 156 that movably supports the same. I do.
- the inspection apparatus is illustrated in FIG. 4 as having only one observation optical system 120A, the inspection apparatus has a plurality of observation optical systems so that a plurality of reaction vessels 101 can be observed simultaneously. Have 120A! /, You may! / ,.
- reaction container 101 to be inspected is placed on the rack 141.
- microplate 142 into which the solution has been dispensed is set in the microplate housing section 144.
- the fitting part 111 is fitted to the target reaction vessel 101 placed on the rack 141 by the XYZ robot 146.
- the fitting section 111 on which the reaction vessel 101 is mounted is moved by the XYZ robot 146, and the reaction vessel 101 is positioned at a position where the determined developer on the microplate 142 can also suck the solution.
- the fitting part 111 on which the reaction vessel 101 is mounted is moved by the XYZ robot 146, and the reaction vessel 101 is placed in the recess 150 of the temperature control unit 147.
- the temperature of the temperature control unit 147 is adjusted by the temperature controller 151 to a temperature suitable for the hybridization reaction.
- the pressure control unit 112 repeatedly pressurizes and depressurizes the inside of the reaction vessel 101 to The liquid is driven up and down through the three-dimensional substrate 102 to cause a hybridization reaction between the sample and the probe in the reaction area.
- the fitting part 111 on which the reaction vessel 101 is mounted is moved by the XYZ robot 146 to position the reaction vessel 101 in the original well of the microplate 142, and the pressure control unit The inside of the reaction vessel 101 is pressurized by 112, and the sample solution is discharged to the original well.
- reaction vessel 101 is positioned by the XYZ robot 146 in the well into which the washing liquid of the microplate 142 has been dispensed.
- the washing liquid is driven an appropriate number of times by repeatedly performing the pressurization and the depressurization in the reaction vessel 101.
- the observation optical system 120A is moved by the XYZ robot 156 so that the observation optical system 120A is fitted to the treated reaction vessel 101 with an upward force, and the fluorescence intensity of the reaction area on the three-dimensional substrate 102 Is detected.
- the hybridization reaction and the detection can be performed separately! Since the processing can be performed sequentially, the experiment and detection for a large number of samples can be performed at high speed.
- the present embodiment is directed to a novel reaction vessel for detecting a biological substance and an apparatus for inspecting a biological substance using the same.
- FIG. 6 schematically shows a reaction container and an inspection device according to a fifth embodiment of the present invention.
- the reaction vessel 171 comprises a three-dimensional base material 172 on which a probe for detecting a biological substance is immobilized, a coupling part 173 coupled to an inspection device, and a solution. And a solution suction part 174 capable of inhaling.
- the three-dimensional base 172 is a member similar to the three-dimensional base 102 of the first embodiment.
- Both the connection part 173 and the solution suction part 174 are made of a resin material containing carbon particles, for example, carbon-containing polypropylene. For this reason, the housing of the reaction vessel 171 (that is, the coupling part 173 and the solution suction part 174) has conductivity.
- the inspection apparatus has a fitting part 181 to which the reaction container 171 is mounted, and an XYZ robot for moving the fitting part 181.
- the fitting portion 181 is conductive and has a voltage measuring electrode.
- the XYZ robot includes an arm 182 supporting the fitting portion 181, a linear motion guide 183 supporting the arm 182 movably in the Z direction, a ball screw 186 engaged with the arm 182, and a ball screw 186. And a control motor 185 for driving the 186.
- the ball screw 186 converts the rotational motion of the control motor 185 into a linear motion of the arm 182 in the Z direction.
- the inspection apparatus further includes a container 191 for storing a solution required for inspection such as a sample solution and a cleaning liquid, and a rack 193 for storing the container 191.
- the container 191 and the rack 193 are both conductive, and the rack 193 has electrodes for voltage measurement.
- the inspection apparatus further includes an AC power supply 201 for applying an AC voltage between the fitting section 181 and the rack 193, a voltmeter 201 for measuring the voltage across the AC power supply 201, and a fitting section. It has an ammeter 205 for measuring the current flowing between the 181 and the rack 193, a motor driver 204 for driving the control motor 185, and a control device 203 for controlling the motor driver 204. I have.
- the control device 203 obtains impedance from the voltage value measured by the voltmeter 201 and the current value measured by the ammeter 205, and performs feedback control of the motor driver 204 based on the impedance.
- the reaction vessel 171 While measuring the impedance between the fitting portion 181 and the rack 193, the reaction vessel 171 is placed in the vessel 191 and lowered toward the liquid surface of the sample solution. [0097] The impedance decreases as the reaction container 171 approaches the liquid surface of the sample solution. When the impedance becomes smaller than the threshold value, the lowering speed of the reaction vessel 171 is reduced.
- the impedance rapidly changes when the reaction vessel 171 comes into contact with the sample solution.
- the reaction vessel 171 is further lowered and stopped from the liquid level to a distance that can suck a predetermined amount of the sample solution. After reaching this position, suction of the sample solution is started by a pressure controller (not shown). If the impedance is monitored, it can be seen that the suction is performed reliably. If the impedance changes abruptly, it means that the suction is defective. For example, the suction can be continued by further lowering the reaction container.
- the reaction vessel 171 comes into contact with the sample solution, the impedance rapidly changes.
- the reaction vessel 171 is further lowered and stopped a predetermined distance from this liquid level. After reaching this position, suction of the sample solution is started by a pressure control unit (not shown). Further, while aspirating the sample solution, the reaction vessel 171 is lowered according to the liquid level movement amount that can be calculated from the suction volume and the capacity of the reaction vessel. At this time, measure the impedance and confirm that the reaction vessel comes into contact with the liquid surface.
- the speed at which the reaction vessel 171 enters the liquid surface can be appropriately controlled by detecting the liquid surface.
- scattering of the solution to be suctioned can be prevented.
- the suction can be performed while checking the liquid level, the solution can be reliably sucked.
- FIG. 7 is a sectional view of an inspection device and a reaction vessel according to a sixth embodiment of the present invention.
- the inspection apparatus includes a fitting section 211 to which the reaction vessel 101 is mounted, a pressure control section 213 that generates a negative pressure, a fitting section 211, and a pressure control section. 213, a pressure control valve 214 provided in the pipe 212, and a pressure measurement for measuring a pressure in the pipe 212 between the pressure control valve 214 and the fitting portion 211. Means 215 and a pressure control device 216 for controlling the pressure control valve 214 based on the information obtained by the pressure measuring means 215.
- a negative pressure is applied to the conduit 212 by the pressure controller 213, and the pressure change in the conduit 212 is measured with a pressure gauge while sucking the sample solution from the sample container 114.
- the pressure S starts to further decrease as shown in FIG. Continue.
- the pressure line 214 is opened to the atmospheric pressure by the pressure control valve 214, and the suction port of the reaction vessel 101 is closed with the plug 217 as shown on the right side of FIG. .
- a further negative pressure is applied, the sample solution passes through the three-dimensional substrate 102 and moves to the top of the three-dimensional substrate 102.
- the sample liquid is then placed under the three-dimensional substrate 102 by opening the pipe 212 to the atmosphere by the pressure control valve 214. Moving.
- the apparatus configuration can be simplified. Further, in the steady state, there is no pressure difference between the two sides of the three-dimensional base material 102, so that the three-dimensional base material 102 is not easily broken.
- FIG. 9 is a sectional view of a reaction vessel according to the seventh embodiment of the present invention.
- the reaction vessel 221 includes a three-dimensional substrate 222 on which a probe for detecting a biological substance is immobilized, and a coupling portion coupled to the fitting portion 111 of the inspection device. 224, a solution suction part 223 capable of sucking the solution, and a filter 225 provided inside the solution suction part 223 for removing dust.
- the three-dimensional substrate 222 is equivalent to the three-dimensional substrate 102 of the first embodiment, and the joints 224 and 223 are equivalent to the joint 103 and the solution suction unit 104 of the first embodiment, respectively. And A detailed description of them will be omitted.
- the filter 225 has a function of filtering the passing solution.
- the solution When the solution is sucked into the reaction vessel 221, the solution is filtered by passing through the filter 225.
- reaction vessel 221 is provided with the filter 225, it is not necessary to filter the solution to remove dust before use.
- the filter 225 preferably has pores having a diameter approximately the same as that of the three-dimensional substrate 222, and more preferably, is formed of the same material. In that case, adhesion of dust to the three-dimensional substrate 222 is more suitably prevented.
- FIG. 10 schematically shows a configuration of the inspection apparatus according to the eighth embodiment of the present invention.
- the members indicated by the above-mentioned reference numerals are substantially the same as the members already explained by the reference numerals, and the detailed description thereof will be omitted.
- the inspection apparatus includes a fitting section 231 to which the reaction vessel 101 is mounted, a pressure control section 234 for generating a positive pressure and a negative pressure, and a fitting section 231.
- Pressure transmission line 232 fluidly connecting the pressure control unit 234, a valve 233 provided in the pressure transmission line 232, a cleaning liquid tank 236 for containing a cleaning liquid, and a cleaning liquid tank.
- a valve 237 provided in the cleaning liquid supply pipe 235.
- the sample container 114 containing the sample solution is set at a predetermined position. With the valve 237 closed, the reaction vessel 101 is mounted on the fitting part 231. The reaction container 101 is lowered toward the sample container 114 by a linear motion mechanism (not shown), and the end of the reaction container 101 is stopped at a position where the solution contained in the sample container 114 can be sucked. A negative pressure is transmitted from the pressure control unit 234 via the pressure transmission pipe 232, and a required amount of the solution is sucked into the reaction vessel 101. The reaction vessel 101 is pulled up from the sample vessel 114 by a linear motion mechanism (not shown). And separate from the solution surface. A positive pressure and a negative pressure are alternately applied by the pressure control unit 234 to move the sample solution up and down the three-dimensional substrate 102 a predetermined number of times.
- a positive pressure is applied by the pressure control unit 234 to move the sample solution under the three-dimensional substrate 102.
- the valve 233 is opened to release the atmospheric pressure
- the valve 237 is opened, and the cleaning liquid tank 236 is pressurized by the pump 239, and the cleaning liquid in the cleaning liquid tank 236 is also supplied by the upward force of the three-dimensional substrate 102.
- the valve 237 is closed, and a positive pressure is applied to the reaction container 101 by the pressure control unit 234 to move the sample solution together with the cleaning liquid below the three-dimensional substrate 102.
- This embodiment is directed to driving the reaction device in the first embodiment. Therefore, the device configuration is the same as in the first embodiment.
- the reaction device and the detection device that constitute the inspection device are configured separately. Therefore, it is necessary to remove the reaction vessel 101 from the fitting part 111 of the reaction device after the reaction is completed.
- the solution when removing the reaction vessel 101, the solution Does not come to the department. For this reason, at the time of imaging by the detection device, an image is taken while the solution is held at the lower part of the reaction vessel 101, and the disturbance of the imaging state due to the liquid level is eliminated. As a result, signals can be obtained with little noise.
- FIG. 11 is a perspective view of the inspection device according to the tenth embodiment of the present invention.
- 12 and 13 show the reaction vessel transport guide shown in FIG. 11, FIG. 12 shows a state where the reaction vessel is housed inside the reaction vessel transport guide, and FIG. 13 shows the reaction vessel transport guide. Is lowered and protrudes from the reaction vessel transport guide.
- the members indicated by the above-mentioned reference numerals are substantially the same as the members already explained by the reference numerals, and the detailed description thereof will be omitted.
- the inspection apparatus includes a reaction vessel rack 242 capable of accommodating a plurality of reaction vessels 101, a reaction vessel transport guide 247 capable of holding the reaction vessels 101, and a reaction vessel rack 242.
- the reaction container transport guide 247 includes a fitting portion 251 to which the reaction container 101 is mounted, an arm 182 supporting the fitting portion 251 and an arm 182. It has a linear motion guide 183 movably supported in the Z direction, a ball screw 186 engaged with the arm 182, and a control motor 185 for driving the ball screw 186.
- the reaction container transport guide 247 includes a rack 261 attached to the arm 182, a pin 262 engaged with the rack 261, a rack 263 engaged with the pin 262, and a rack 263. It has a solution receiver 265 connected to the lower end of the 263 via a hinge 264, and a pin 266 for guiding the solution receiver 265.
- the reaction container 101 attached to the fitting part 251 is moved up and down by the control motor 185 as in the fifth embodiment.
- the rack 261 attached to the arm 182 supporting the fitting part 251 also moves up and down in conjunction with the vertical movement of the fitting part 251.
- the rack 263 moves up and down in the opposite direction to the rack 261.
- Rack 263 In conjunction with the upward and downward movement of the solution receiver 265, the connection part of the solution receiver 265 with the hinge 264 moves up and down while being guided by the pin 266.
- the solution receiver 265 is preferably shaped so that the contained solution does not spill.
- Solution receiver 265 preferably has an absorbing member that absorbs and holds the contained solution. Also, the solution receiver 265 is easily replaceable.
- the inspection device since the solution dripping from the reaction vessel 101 is stored in the solution receiver 265, the inspection device is not contaminated with the solution.
- FIG. 14 schematically shows the configuration of the inspection apparatus according to the eleventh embodiment of the present invention.
- FIG. 15 is a plan view of the fitting portion shown in FIG. 14 as viewed from below.
- a fitting portion 271 to which the reaction vessel 101 is attached includes an observation optical system for optically observing the three-dimensional substrate 102.
- the fitting portion 271 includes an imaging lens 272 for forming an optical image of the three-dimensional substrate 102 and a three-dimensional image formed by the imaging lens 272 as shown in FIGS. A CCD 273 for converting an optical image of the substrate 102 into an electric signal.
- the inspection device has an image capturing device 274 that captures a signal from the CCD 273 and converts the signal into digital data.
- the fitting portion 271 includes an illumination optical system 276 that emits light for exciting the fluorescent molecules remaining on the three-dimensional substrate 102.
- the inspection apparatus fluidly connects the pressure control unit 279 for generating positive pressure and negative pressure, the fitting unit 271 and the pressure control unit 279, and Pressure transmission Pipe 278, a valve 280 provided in the pressure transmission pipe 278, a cleaning liquid tank 282 for containing a cleaning liquid, a pump 285 for pressurizing the cleaning liquid tank 282, a cleaning liquid tank 282 and a pump 285.
- Tube 284 fluidly connecting the cleaning fluid supply pipe 281 fluidly connecting the fitting portion 271 and the cleaning fluid tank 282, and the knob provided in the cleaning fluid supply pipeline 281. 283, and a cleaning nozzle 286 provided at an end of the cleaning liquid supply pipe 281!
- the reaction container 101 is attached to the fitting portion 271.
- a negative pressure is generated by the pressure control unit 279, the knob 280 is opened, and the sample solution (not shown) is also drawn into the reaction container 101.
- a positive pressure and a negative pressure are alternately applied by the pressure control unit 279 to drive the sample solution up and down the three-dimensional substrate 102.
- the knob 280 is opened to release the reaction vessel 101 to the atmospheric pressure.
- the valve 283 is opened, the cleaning solution tank 282 is pressurized by the cleaning solution pump 285, and the cleaning solution is sent from the cleaning solution tank 282 to the fitting portion 271.
- the cleaning liquid sent to the fitting portion 271 is jetted by the cleaning nozzle 286 to the lower end portion of the fitting portion 271 to clean the lower end portion of the fitting portion 271.
- valve 283 After washing, the valve 283 is closed. Further, the valve 280 is opened, and a positive pressure is generated by the pressure control unit 279 to move the cleaning liquid under the three-dimensional substrate 102. After that, an image is acquired by the CCD273.
- the imaging lens 272 even if the imaging lens 272 becomes cloudy or dirty, it is possible to stably shoot by cleaning the imaging lens 272.
- FIG. 16 schematically shows the configuration of the inspection apparatus according to the twelfth embodiment of the present invention.
- the inspection apparatus measures the fitting portion 111 to which the reaction vessel 101 is mounted, the heater 291 for controlling the temperature of the reaction vessel 101, and the temperature of the heater 291. And a temperature controller 293 for controlling the temperature of the heater 291 based on the information obtained by the temperature sensor 292.
- housing or coupling portion 103 and the solution sucking portion 104 of the reaction vessel 101 is composed of PP, the linear expansion coefficient of about 6 X 10- 5.
- the fitting portion 111 is composed of high density PE, linear expansion coefficient is about 1 X 10- 4. That is, the linear expansion coefficient of the fitting portion 111 is larger than that of the coupling portion 103 of the reaction vessel 101.
- the connecting portion 103 of the reaction vessel 101 expands, and the diameter of the opening end increases.
- the linear expansion coefficient of the fitting part 111 is larger than that of the coupling part 103, the fitting part 111 expands more than the expansion of the opening end.
- the space between the reaction vessel 101 and the fitting portion 111 is kept airtight.
- FIG. 17 schematically shows the configuration of the inspection apparatus according to the thirteenth embodiment of the present invention.
- the members indicated by the above-mentioned reference numerals are substantially the same as the members already explained by the reference numerals, and the detailed description thereof will be omitted.
- the inspection device includes a fitting portion 301 to which the reaction vessel 101 is mounted, and a heater for controlling the temperature of the fitting portion 301.
- the temperature of the heater 291 is controlled based on the information obtained by the temperature sensor 303 and the temperature sensor 303 for measuring the temperature of the fitting portion 301, and the temperature of the heater 291 is controlled based on the information obtained by the temperature sensor 303.
- housing or coupling portion 103 and the solution sucking portion 104 of the reaction vessel 101 is constituted by PP
- the linear expansion coefficient is approximately 6 X 10- 5 .
- Fitting section 301 is composed of stainless steel, its linear expansion coefficient is about 7 X 10- 6. Therefore, the linear expansion coefficient of the fitting portion 301 is smaller than that of the connecting portion 103 of the reaction vessel 101.
- the temperature of the fitting portion 301 is constantly controlled by the temperature control device 304 to be higher than the temperature of the reaction vessel 101.
- the temperature of the fitting portion 301 and the temperature of the coupling portion 103 of the reaction vessel 101 are adjusted so that the amounts of thermal expansion thereof are substantially the same.
- gene hybridization In order to control the temperature T to the optimum temperature for the reaction, the temperature of the reaction vessel 101 is controlled to T ° C by the temperature controller 304. Further, the temperature of the fitting portion 301 is controlled to be 10 ° C. higher than the temperature of the reaction vessel 101 by the temperature control device 304.
- the temperature of the fitting section 301 and the joining section 103 is controlled by the temperature control device 304 so that the amounts of thermal expansion of the joining section 301 and the joining section 103 are substantially the same. Good airtightness is maintained between 103 and the fitting portion 301.
- FIG. 18 schematically shows the configuration of the inspection apparatus according to the fourteenth embodiment of the present invention.
- the members indicated by the above-mentioned reference numerals are substantially the same as the members already explained by the reference numerals, and the detailed description thereof will be omitted.
- the inspection apparatus measures the fitting portion 301 to which the reaction vessel 101 is mounted, the heater 291 for controlling the temperature of the reaction vessel 101, and the temperature of the heater 291. And a temperature controller 293 for controlling the temperature of the heater 291 based on the information obtained by the temperature sensor 292.
- the housing of the reaction vessel 101 that is, the coupling part 103 and the solution suction part 104 are made of PP, and the fitting part 311 is made of stainless steel.
- the fitting portion 311 has an inner fitting surface facing the inner surface of the coupling portion 103 of the reaction vessel 101, and an outer fitting surface facing the outer surface of the coupling portion 103 of the reaction vessel 101.
- the reaction container 101 from which the sample solution has been sucked by the pressure control unit (not shown) is set in the heater 291.
- the target temperature is set in the temperature controller 293.
- the temperature control device 293 conducts electricity to the heater 291 until the temperature reaches the set temperature based on the temperature information from the temperature sensor 292.
- the temperature of the reaction vessel 101, the sample solution, and the fitting section 311 are simultaneously controlled by the heat conduction from the housing of the reaction vessel 101, that is, the coupling section 103 and the solution suction section 104.
- the joint 103 of the reaction vessel 101 expands. Due to the expansion, the joint 103 has an increased wall thickness. Also, due to the difference in linear expansion coefficient between the joint 103 and the fitting 311, The inner surface of 103 also tends to separate the inner fitting surface force of the fitting portion 311. However, before the inner surface of the connecting portion 103 separates from the inner fitting surface force of the fitting portion 311, the outer surface of the connecting portion 103 fits due to an increase in the diameter of the opening end of the connecting portion 103 and an increase in the wall thickness.
- the joint 103 and the fitting 311 are arranged such that the outer surface of the joint 103 is on the outer fitting surface of the fitting 311 before the inner surface of the joint 103 is separated from the inner fitting surface of the fitting 311. Designed to make contact.
- the space between the coupling part 103 and the fitting part 311 of the reaction vessel 101 is always kept airtight.
- FIG. 19 is a plan view schematically showing the configuration of the inspection apparatus according to the fifteenth embodiment of the present invention.
- FIG. 20 schematically shows a cross section of the turntable shown in FIG.
- FIG. 21 schematically illustrates the sample collection device shown in FIG.
- FIG. 22 schematically shows a cross section of a peripheral portion of the reaction container supply device shown in FIG.
- the inspection device 320 includes a sample supply unit 322, a reaction vessel supply device 323, a sample sump collection device 325, a turn tape notch 324, a first solution rack 326, A single dispenser 327, a second solution rack 328, a second dispenser 329, and a detector 330 are provided.
- the sample supply unit 322 sequentially supplies a rack 321 containing a plurality of sample containers into which a sample solution has been dispensed, for inspection.
- the reaction vessel supply device 323 stores a plurality of reaction vessels 101, and supplies the reaction vessels 101 one by one by the arm 361.
- the turntable 324 has a plurality of reaction container housing portions 337 arranged on the circumference. More specifically, as shown in FIG. 20, the turntable 324 includes a rotating body 334 holding a plurality of reaction vessel housing portions 337 and a drive for rotating the rotating body 334 with respect to the base 331. A part 332 is provided.
- Each reaction container storage section 337 has a storage space for storing the reaction container 101, and The space is fluidly coupled to a pressure source, not shown, located below the base 331 via piping. Further, the reaction container housing section 337 has a lid 338 that can be opened and closed, and the lid 338 has an optical window 339 that enables optical detection from above by the detection device 330.
- the turntable 324 further includes a lid opening / closing mechanism 341 for opening and closing the lid 338 of the reaction container housing portion 337, and a fixed disk 335 supporting the lid opening / closing mechanism 341.
- the fixed disk 335 is fixed to the base 331 and does not rotate.
- the lid opening / closing mechanism 341 is provided at a working position of the sample collecting device 325, the first dispensing device 327, and the second dispensing device 329.
- the sample collecting device 325 supports a fitting portion 351 to which the reaction vessel 101 is mounted, an arm 352 supporting the fitting portion 351, and an arm 352. It has a supporting column 353, and the supporting column 353 can move up and down and rotate with respect to the base 354 by a driving mechanism (not shown). Therefore, the sample collection device 325 can mount the reaction container 101 supplied from the reaction container supply device 323 to the fitting portion 351 by the vertical movement and rotation of the arm 352 supporting the fitting portion 351. It is. Although not particularly shown, the sample collecting device 325 also has a mechanism for removing the reaction container 101 attached to the fitting portion 351.
- the fitting portion 351 is fluidly connected to the pressure control portion via a pipe line, as in the previous embodiments.
- the positive pressure and the negative pressure can be supplied to the reaction container 101 mounted on the fitting portion 351.
- the sample collection device 325 receives the reaction container 101 supplied from the reaction container supply device 323, moves the reaction container 101 around the sample supply unit 322, and reacts the sample solution.
- the reaction container 101 containing the sample solution is sucked into the container 101, moved to the turntable 324, and the reaction container 101 can be supplied to the reaction container container 337.
- the first solution rack 326 and the second solution rack 328 have substantially the same structure, and store solutions required for inspection. For example, a container in which reagents necessary for the test are dispensed is stored at an appropriate temperature and humidity, and a container for the necessary reagents is placed at a suction position.
- the first dispensing device 327 and the second dispensing device 329 have substantially the same structure, The solution may be dispensed from the first solution rack 326 and the second solution rack 328 into the reaction vessel 101.
- the detection device 330 includes, for example, a fluorescence microscope, and can take a fluorescence image of a three-dimensional substrate in the reaction vessel 101.
- the inspection device 320 of the present embodiment operates, for example, as follows.
- the reaction container 101 supplied from the reaction container supply device 323 is attached to the fitting portion 351 of the sample collection device 325.
- the sample collection device 325 sucks the sample solution from the sample rack 321 of the sample supply unit 322 into the reaction container 101, and places the reaction container 101 into which the sample solution has been sucked into the reaction container storage unit 337 of the turntable 324. Deploy. Thereafter, the lid 338 of the reaction container housing part 337 is closed by the lid opening / closing mechanism 341.
- reaction container 101 accommodated in the container accommodating portion 337 passes through the first dispensing device 327, the second dispensing device 329, and the detecting device 330 in order by rotation of the turntable 324, and finally Return to the sampling device 325 again.
- reaction vessel 101 While the reaction vessel 101 is being sent from the sample collection device 325 to the first dispensing device 327, positive and negative pressures are repeatedly applied to the reaction vessel storage section 337 to cause the sample solution in the reaction vessel 101 to move. To drive the complementary binding reaction.
- the lid 338 of the reaction container housing part 337 is opened by the lid opening / closing mechanism 341.
- the washing solution is dispensed into the reaction vessel 101 by the first dispensing device 327, and the sample solution is washed away by repeatedly applying a positive pressure and a negative pressure to the reaction vessel housing part 337.
- the lid 338 of the reaction container housing part 337 is closed by the lid opening / closing mechanism 341.
- the lid 338 of the reaction container housing part 337 is opened by the lid opening / closing mechanism 341.
- the luminescent substrate is dispensed into the reaction vessel 101 by the second dispensing device 329, and the positive pressure and the negative pressure are repeatedly applied to the reaction vessel accommodating portion 337 to promote the reaction. Thereafter, the luminescent substrate is washed away with the washing liquid, and the lid 338 of the reaction container housing part 337 is closed by the lid opening / closing mechanism 341.
- reaction vessel 101 reaches the detection device 330, an image of the three-dimensional substrate in the reaction container 101 is captured by the detection device 330, and the brightness of each spot on the three-dimensional substrate is determined by image analysis software. Is measured.
- sample collection device 325 removes the reaction container 101 from the reaction container accommodating section 337 of the turntable 324, and disposes the waste container as shown in FIG. Discard in hole 363.
- an apparatus for handling the reaction vessel 101 becomes unnecessary, so that the inspection apparatus can be made compact.
- the present embodiment is directed to a method for manufacturing a novel reaction container for detecting a biological substance which appears in the embodiments described above.
- description will be made assuming that a nylon filter is applied to a three-dimensional base material.
- a square nylon filter 441 is prepared, and a mark 442 is formed on a part of the outer periphery.
- a nylon filter 441 is arranged on a stage 461 of the inkjet printer. At this time, the nylon filter 441 is applied to the application section 462 on the stage 461 for positioning. When attaching the nylon filter 441 to the attaching section 462, the direction of the nylon filter 441 is determined by the mark 442.
- nucleic acid probes 443 are spotted at predetermined positions of the nylon filter 441 by an ink jet printer to form spot regions 444.
- spot regions 444 a three-dimensional substrate 440 on which the probe is immobilized is produced.
- the spot diameter is adjusted to 100 ⁇ m and the spot interval is adjusted to 200 ⁇ m.
- the solution suction unit main body 410 is applied to the application jig 463 and positioned.
- the solution suction portion main body 410 is composed of a plate-shaped portion 411 having a notch 414 at one corner and a truncated cone 412 protruding from the plate-shaped portion 411, and penetrates the plate-shaped portion 411 and the truncated cone 412. Has a through hole 413.
- an acrylic adhesive 451 (see Fig. 28) is applied to the upper surface of the plate-shaped portion 411 of the solution suction portion main body 410 applied to the application jig 463 in this manner, and the tertiary prepared above is applied.
- the original base material 440 is positioned by applying an abutment jig 463 to the abutment jig, and attached to the upper surface of the plate-shaped portion 411 of the solution suction portion main body 410. Apply 3D base material 440 to application jig 463 At this time, the orientation of the three-dimensional substrate 440 is determined by the relative position of the mark 442 with respect to the notch 414 of the plate-shaped portion 411.
- the three-dimensional substrate 440 is always attached to the solution suction unit main body 410 in the same direction.
- the spot area 444 is located inside the through hole 413. Since the plate-shaped part 411 of the solution suction part main body 410 and the three-dimensional base material 440 are bonded by bonding, the airtightness between them is maintained.
- the coupling section 430 is attached to the solution suction section main body 410.
- the connecting portion 430 also becomes a plate-like member, has a notch 434 at one corner, and has a through hole 433 at the center.
- the connecting portion 430 is almost the same size as the plate-shaped portion 411 of the solution suction portion main body 410, and when the connecting portion 430 and the plate-shaped portion 411 are properly combined, the respective cutout portions 434 and 414 are aligned. It's like that.
- An acrylic adhesive 452 (see FIG. 28) is applied to the plate-shaped portion 411 of the solution suction portion main body 410 and the three-dimensional base material 440 at appropriate positions, and the cutout portion 434 of the joint portion 430 is attached to the solution suction portion main body. Align the notch 414 of the 410 with the notch 414, position the joint 430 against the application jig 463, and attach it to the solution suction unit main body 410. Since the three-dimensional base material 440 and the joint 430 are joined by bonding, the airtightness between them is maintained.
- R1 indicates the inner diameter of the through-hole 433 of the joint 430
- R2 indicates the maximum distance of the spot area 444 of the three-dimensional substrate 440
- R3 indicates the inner diameter of the through-hole 413 of the solution suction part main body 410.
- R3 which satisfy the relationship of R3> R1> R2.
- the present embodiment is directed to another method for manufacturing a reaction container.
- the manufacturing method of the present embodiment will be described with reference to FIGS.
- members denoted by the same reference numerals as those in the sixteenth embodiment are the same members, and detailed description thereof will be omitted.
- a joint 430 is prepared, an acrylic adhesive is applied to an appropriate position of the joint 430, and a square nylon filter 441 is joined so as to cover the through hole 433. Attach to part 430. Since the nylon filter 441 is bonded to the bonding portion 430 with an acrylic adhesive, the airtightness between the two is maintained.
- the joint 430 to which the nylon filter 441 is attached is placed on the stage 465 of the inkjet printer.
- the connecting portion 430 is applied to the abutting portion 466 on the stage 465 for positioning.
- the orientation of the connecting portion 430 is determined by the cutout portion 434.
- nucleic acid probes are spotted at predetermined positions of the nylon filter 441 by an ink jet printer to form spot areas.
- a three-dimensional substrate 440 on which the probe is immobilized is produced.
- the spot diameter is adjusted to 100 m and the spot interval is adjusted to 200 ⁇ m.
- the solution suction unit main body 410 is applied to the application jig 463 and positioned.
- the orientation of the solution suction unit main body 410 is determined by the notch 414.
- an acrylic adhesive 452 is applied to an appropriate position of the plate-shaped portion 411 of the solution suction portion main body 410, and the cutout portion 434 of the connection portion 430 is aligned with the cutout portion 414 of the solution suction portion main body 410 to be connected.
- the part 430 is applied to the application jig 463 for positioning, and attached to the solution suction part main body 410. Since the three-dimensional base material 440 and the solution suction part main body 410 are bonded by bonding, airtightness between them is maintained.
- reaction container manufactured in the present embodiment a mark is formed on the nylon filter 441. Except that it is not formed, it is the same as the reaction container manufactured in the sixteenth embodiment.
- the present embodiment is directed to another method for manufacturing a reaction container.
- the manufacturing method of this embodiment will be described with reference to FIGS.
- members denoted by the same reference numerals as those in the sixteenth embodiment are the same members, and detailed description thereof will be omitted.
- a solution suction unit main body 410 is prepared, and an acrylic adhesive is applied to an appropriate position of the plate-shaped portion 411 of the solution suction unit main body 410 so as to cover the through-hole 413. Then, a square nylon filter 441 is attached to the solution suction part main body 410. Since the nylon filter 441 is connected to the solution suction portion main body 410 by an acrylic adhesive, the airtightness between the two is maintained.
- the solution suction part main body 410 to which the nylon filter 441 is attached is placed on the stage 467 of the ink jet printer.
- the solution suction unit main body 410 is applied to the application unit 468 on the stage 467 for positioning.
- the orientation of the solution suction unit main body 410 is determined by the notch 413.
- nucleic acid probes are spotted at predetermined positions of the nylon filter 441 by an ink jet printer to form spot areas.
- a three-dimensional substrate 440 on which the probe is immobilized is produced.
- the spot diameter is adjusted to 100 m and the spot interval is adjusted to 200 ⁇ m.
- the solution suction unit main body 410 is applied to the application jig 463 and positioned.
- the orientation of the solution suction unit main body 410 is determined by the notch 414.
- an acrylic adhesive 452 is applied to the plate-shaped part 411 of the solution suction part main body 410 and the three-dimensional base material 440 at appropriate positions, and the cutout part 434 of the joint part 430 is cut out 414 of the solution suction part main body 410.
- the connecting portion 430 is positioned by applying a contact jig 463 to the solution suction portion main body 410.
- the reaction container manufactured in the present embodiment is the same as the reaction container manufactured in the sixteenth embodiment, except that no mark is formed on the nylon filter 441.
- an acrylic adhesive was used for joining the nylon filter 441 to the solution absorbing portion main body 410 and joining the nylon filter 441 to the joining portion 430.
- applied means other than the acrylic adhesive, for example, ultrasonic welding, heat welding, laser welding and the like may be applied.
- the present embodiment is directed to another method for manufacturing a reaction container.
- the manufacturing method of this embodiment will be described with reference to FIGS.
- a square nylon filter 541, a protection member 542, and a protection member 545 are prepared.
- the protection member 542 is a rectangular thin plate member having a cutout 543 at one corner and a circular opening 544 at the center.
- the protection member 545 is a rectangular thin plate member having a cutout 546 at one corner and a circular opening 547 at the center. 36, the protective member 542 is slightly larger than the protective member 545, and the opening 544 of the protective member 542 is slightly smaller than the opening 547 of the protective member 545.
- an acrylic adhesive 548 (see FIG. 36) is applied to a proper position on the lower surface of the protective member 542, and an acrylic adhesive 549 (see FIG. 36) is applied to a proper position on the upper surface of the protective member 545.
- the protective member 542 and the protective member 545 are bonded together with the nylon filter 541 interposed therebetween.
- the three-dimensional base chip 540 before the formation of the probe spot is manufactured. Since the nylon filter 541 and the protection member 542 are bonded by bonding, the airtightness between them is maintained. Similarly, the airtightness between the nylon filter 541 and the protection member 545 is maintained.
- the three-dimensional base material chip 540 prepared above is placed on the stage 561 of the inkjet printer with the protective member 542 facing upward. At this time, the three-dimensional base chip 540 is applied to the application section 562 on the stage 561 for positioning.
- the orientation of the three-dimensional base material chip 540 is determined by the cutout part 543 of the protection member 542.
- the probe is immobilized on the nylon filter 541 of the three-dimensional substrate chip 540.
- the spot diameter is adjusted to 100 ⁇ m and the spot interval is adjusted to 200 ⁇ m.
- the solution suction portion main body 510 includes a plate-shaped portion 511 having a notch 515 at one corner, and a truncated cone portion 512 protruding from the plate-shaped portion 511. It has a through hole 513 penetrating the truncated cone portion 512.
- the plate-shaped portion 511 has a concave portion 514 that can accommodate the three-dimensional substrate chip 540.
- the concave portion 514 has application surfaces 514a and 514b to which two sides of the three-dimensional base chip 540 are applied.
- the concave portion 514 corresponds to the outer shape of the three-dimensional base chip 540, and has a hypotenuse portion 514c at one corner.
- the slope portion 514c is located near the notch 515.
- the plate-shaped portion 511 has four screw holes 516 for screwing a coupling portion 530 described later at four corners.
- the O-ring 551 is arranged on the bottom surface of the concave part 514 of the solution suction part main body 510, and the three-dimensional base chip 540 is disposed thereon. It is performed by placing.
- the connecting portion 530 shown in FIG. 39 is attached to the solution suction portion main body 510.
- the connecting portion 530 also has a force with the plate portion 531 and the cylindrical portion 532 protruding from the plate portion 531, and a through hole 533 penetrating the plate portion 531 and the cylindrical portion 532. have.
- the plate portion 531 has a through hole 536 through which a screw 555 for fixing the coupling portion 530 to the solution suction portion main body 510 passes.
- Attachment of the connecting portion 530 to the solution suction unit main body 510 is performed by disposing an O-ring 552 (see Fig. 40) on the three-dimensional base chip 540 housed in the concave portion 514 of the solution suction unit main body 510.
- the screw 555 is passed through the through holes 536 at the four corners of the plate portion 531 of the connecting portion 530 and tightened into the screw holes 516 at the four corners of the plate portion 511 of the solution suction portion main body 510.
- the three-dimensional base chip 540 is in contact with the solution suction part main body 510, and the three-dimensional base chip 540 is in contact with the solution suction part main body 510 via the O-ring 551 or the gasket, so that the space between the three-dimensional base chip 540 and the solution suction part main body 510 is airtight.
- the three-dimensional base chip 540 is held in contact with the joint 530 via the O-ring 552, so that the space between the three-dimensional base chip 540 and the joint 530 is held airtight.
- R1 indicates the inner diameter of the through hole 533 of the coupling portion 530
- R2 indicates the inner diameter of the opening 544 of the protection member 542 of the three-dimensional substrate chip 540
- R3 indicates the maximum distance of the spot area 544
- R 4 indicates the inner diameter of the opening 547 of the protection member 545
- R5 indicates the inner diameter of the through hole 513 of the solution suction part main body 510, which satisfies R1> R2, R4> R2, and R5> R4.
- the O-ring 551 connects between the three-dimensional base chip 540 and the solution suction part main body 510, and the O-ring between the three-dimensional base chip 540 and the joint 530. 552 can be kept more airtight.
- reaction container manufactured in the present embodiment is substantially the same as the reaction container manufactured in the sixteenth embodiment.
- the members forming the reaction vessel are fixed with an adhesive or a fitting screw.
- the fixing method is to keep the solution in an airtight state so that the solution can be sucked and discharged into the reaction vessel. You will not be limited to these if you fall.
- a tapered cylindrical body is fitted to the truncated cone of the solution suction unit main body or screwed. If it is made removable, the tapered tubular body can be removed after the completion of the reaction and washing steps to perform detection. This is particularly effective when the reaction device and the detection device are separate, and the size of the detection device can be reduced. Also, if the joint is removed from the plate, there will be no parts that interfere with the three-dimensional substrate, so scanning multiple plate-like parts will enable faster detection of the reaction results. Become.
- a fluorescent dye is used as a label for a biological substance.
- various detection methods and labels can be applied to the present invention.
- a light source for illuminating the sample is not required because light is emitted by the reaction between the enzyme and the substrate.
- various fluorescent substances can be used as labels, and fluorescent glass particles and the like can be used in addition to various fluorescent dyes.
- metal particles or dielectric particles are used as the labels. For example, fine particles of gold, silver, platinum, silicon and the like, or latex particles can be used.
- fine particles of a metal such as gold, silver, and platinum are particularly preferably those having a particle size of 10 to 100 nm, because the speed of the particles in a moving state is optimal.
- latex particles having a particle diameter of 0. 0 m are particularly preferable because the speed of the particles in the moving state is also optimal.
- the appropriate particle size is determined by the specific gravity of the particles and the speed of Brownian motion.
- the motion state of the particles includes, for example, Brownian motion and vibration.
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- Health & Medical Sciences (AREA)
- Chemical & Material Sciences (AREA)
- Clinical Laboratory Science (AREA)
- Chemical Kinetics & Catalysis (AREA)
- Analytical Chemistry (AREA)
- General Health & Medical Sciences (AREA)
- Life Sciences & Earth Sciences (AREA)
- Physics & Mathematics (AREA)
- Hematology (AREA)
- Biochemistry (AREA)
- General Physics & Mathematics (AREA)
- Immunology (AREA)
- Pathology (AREA)
- Apparatus Associated With Microorganisms And Enzymes (AREA)
- Automatic Analysis And Handling Materials Therefor (AREA)
- Investigating Or Analysing Biological Materials (AREA)
Abstract
Description
Claims
Priority Applications (3)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
JP2005516000A JPWO2005054844A1 (ja) | 2003-12-04 | 2004-12-03 | 反応容器およびそれを利用する反応装置および検出装置および反応容器の作製方法 |
EP04819948A EP1693670A4 (en) | 2003-12-04 | 2004-12-03 | REACTION CONTAINER AND REACTION DEVICE CONTAINING SAME, DETECTION DEVICE AND METHOD FOR PRODUCING THE REACTION CONTAINER |
US11/445,999 US20060275892A1 (en) | 2003-12-04 | 2006-06-02 | Reaction vessel, reaction apparatus and detection apparatus using the same, and method of manufacturing reaction vessel |
Applications Claiming Priority (2)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
JP2003-405789 | 2003-12-04 | ||
JP2003405789 | 2003-12-04 |
Related Child Applications (1)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
US11/445,999 Continuation US20060275892A1 (en) | 2003-12-04 | 2006-06-02 | Reaction vessel, reaction apparatus and detection apparatus using the same, and method of manufacturing reaction vessel |
Publications (1)
Publication Number | Publication Date |
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WO2005054844A1 true WO2005054844A1 (ja) | 2005-06-16 |
Family
ID=34650234
Family Applications (1)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
PCT/JP2004/018063 WO2005054844A1 (ja) | 2003-12-04 | 2004-12-03 | 反応容器およびそれを利用する反応装置および検出装置および反応容器の作製方法 |
Country Status (4)
Country | Link |
---|---|
US (1) | US20060275892A1 (ja) |
EP (1) | EP1693670A4 (ja) |
JP (1) | JPWO2005054844A1 (ja) |
WO (1) | WO2005054844A1 (ja) |
Cited By (4)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
JP2006345813A (ja) * | 2005-06-17 | 2006-12-28 | Toppan Printing Co Ltd | 反応容器および反応方法 |
JP2007081390A (ja) * | 2005-08-17 | 2007-03-29 | Nikon Corp | 観察装置、計測装置、露光装置及び露光方法、並びにデバイス製造方法、デバイス製造用基板、位置決め装置 |
US8895296B2 (en) | 2008-12-25 | 2014-11-25 | Hitachi High-Technologies Corporation | Analyzer |
JP2017138306A (ja) * | 2016-01-31 | 2017-08-10 | アークレイ株式会社 | 分析用具および分析装置 |
Families Citing this family (9)
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JP4043859B2 (ja) * | 2002-06-18 | 2008-02-06 | 浜松ホトニクス株式会社 | 樹脂溶接装置及び樹脂溶接方法 |
US20060132153A1 (en) * | 2004-12-22 | 2006-06-22 | Formfactor, Inc. | Assembly with a detachable member |
JP4853358B2 (ja) * | 2007-03-30 | 2012-01-11 | 株式会社日立プラントテクノロジー | 発光測定装置 |
US9116129B2 (en) * | 2007-05-08 | 2015-08-25 | Idexx Laboratories, Inc. | Chemical analyzer |
US20090017554A1 (en) * | 2007-06-28 | 2009-01-15 | Applera Corporation | Detection and mixing in a conduit in integrated bioanalysis systems |
JP4811797B2 (ja) * | 2010-01-26 | 2011-11-09 | 株式会社日立プラントテクノロジー | 発光測定装置の配管洗浄方法、発光測定装置の配管洗浄機構 |
WO2016132945A1 (ja) * | 2015-02-20 | 2016-08-25 | コニカミノルタ株式会社 | 反応方法および反応装置 |
JP6676300B2 (ja) * | 2015-07-28 | 2020-04-08 | ヤマハ発動機株式会社 | 対象物移動方法及び装置 |
US11977091B2 (en) | 2020-07-10 | 2024-05-07 | Idexx Laboratories Inc. | Point-of-care medical diagnostic analyzer and devices, systems, and methods for medical diagnostic analysis of samples |
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WO2003027673A1 (fr) * | 2001-07-31 | 2003-04-03 | Olympus Corporation | Appareil d'inspection genique et procede d'extraction d'acide nucleique cible faisant appel a cet appareil |
JP2003344401A (ja) * | 2002-05-30 | 2003-12-03 | Olympus Optical Co Ltd | 生体関連物質の検査方法 |
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EP0561003A1 (en) * | 1991-11-19 | 1993-09-22 | La Mina Ltd. | Device for detecting disease markers |
CA2105962A1 (en) * | 1992-09-18 | 1994-03-19 | Margaret Patricia Raybuck | Device and method for affinity separation |
US6660233B1 (en) * | 1996-01-16 | 2003-12-09 | Beckman Coulter, Inc. | Analytical biochemistry system with robotically carried bioarray |
US7025876B2 (en) * | 2001-09-17 | 2006-04-11 | Hitachi, Ltd. | Sample processing device and sample processing method |
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2004
- 2004-12-03 JP JP2005516000A patent/JPWO2005054844A1/ja active Pending
- 2004-12-03 EP EP04819948A patent/EP1693670A4/en not_active Withdrawn
- 2004-12-03 WO PCT/JP2004/018063 patent/WO2005054844A1/ja active Application Filing
-
2006
- 2006-06-02 US US11/445,999 patent/US20060275892A1/en not_active Abandoned
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WO2003027673A1 (fr) * | 2001-07-31 | 2003-04-03 | Olympus Corporation | Appareil d'inspection genique et procede d'extraction d'acide nucleique cible faisant appel a cet appareil |
JP2003344401A (ja) * | 2002-05-30 | 2003-12-03 | Olympus Optical Co Ltd | 生体関連物質の検査方法 |
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Cited By (5)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
JP2006345813A (ja) * | 2005-06-17 | 2006-12-28 | Toppan Printing Co Ltd | 反応容器および反応方法 |
JP2007081390A (ja) * | 2005-08-17 | 2007-03-29 | Nikon Corp | 観察装置、計測装置、露光装置及び露光方法、並びにデバイス製造方法、デバイス製造用基板、位置決め装置 |
US8895296B2 (en) | 2008-12-25 | 2014-11-25 | Hitachi High-Technologies Corporation | Analyzer |
US9523114B2 (en) | 2008-12-25 | 2016-12-20 | Hitachi High-Technologies Corporation | Analyzer |
JP2017138306A (ja) * | 2016-01-31 | 2017-08-10 | アークレイ株式会社 | 分析用具および分析装置 |
Also Published As
Publication number | Publication date |
---|---|
JPWO2005054844A1 (ja) | 2007-12-06 |
US20060275892A1 (en) | 2006-12-07 |
EP1693670A1 (en) | 2006-08-23 |
EP1693670A4 (en) | 2008-06-11 |
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