WO2019188304A1 - Dispositif de détection - Google Patents

Dispositif de détection Download PDF

Info

Publication number
WO2019188304A1
WO2019188304A1 PCT/JP2019/010348 JP2019010348W WO2019188304A1 WO 2019188304 A1 WO2019188304 A1 WO 2019188304A1 JP 2019010348 W JP2019010348 W JP 2019010348W WO 2019188304 A1 WO2019188304 A1 WO 2019188304A1
Authority
WO
WIPO (PCT)
Prior art keywords
light guide
excitation light
light
fluorescence
axis
Prior art date
Application number
PCT/JP2019/010348
Other languages
English (en)
Japanese (ja)
Inventor
智和 酒井
陽平 松葉
Original Assignee
パイオニア株式会社
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by パイオニア株式会社 filed Critical パイオニア株式会社
Priority to JP2020509875A priority Critical patent/JP6992164B2/ja
Publication of WO2019188304A1 publication Critical patent/WO2019188304A1/fr

Links

Images

Classifications

    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/62Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
    • G01N21/63Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
    • G01N21/64Fluorescence; Phosphorescence

Definitions

  • the present invention relates to a detection apparatus for detecting a substance contained in a gas sample.
  • a detection device that detects a specific substance contained in a gas sample by detecting a decrease in coenzyme accompanying an enzyme reaction is known.
  • the detection of a substrate contained in a gas sample can be performed by using a decrease in NADH which is a coenzyme with the reaction of a ketone such as acetone or a substrate such as nonenal.
  • a biosensor system to be performed is disclosed in Patent Document 1. Specifically, the biosensor system of Patent Document 1 detects a decrease in coenzyme by using fluorescence when the specific enzyme is irradiated with specific excitation light.
  • the amount of fluorescence emitted by the coenzyme affects the detection accuracy. Therefore, in order to increase the amount of detectable fluorescence, it is conceivable to efficiently irradiate the coenzyme with excitation light emitted from the light source and efficiently guide only the fluorescence emitted by the coenzyme to the detection unit. For this reason, in the biosensor system of Patent Document 1, an optical fiber probe is arranged in the vicinity of an enzyme in which the concentration of the coenzyme changes due to the substrate, through which the coenzyme is irradiated with excitation light, and the coenzyme The fluorescence emitted from is detected.
  • NA numerical aperture
  • the detection device when the detection device is mounted on a moving body such as an automobile, the mounting space is limited. For this reason, the detection device is required to be reduced in size by reducing the number of parts.
  • the present invention has been made in view of the above points, and is a detection device capable of improving the detection accuracy of a specific substance by improving the utilization efficiency of excitation light and fluorescence and reducing the size of the device. Is one of the issues.
  • the detection device is a solution that holds a solution containing a coenzyme that emits fluorescence by being excited by excitation light before or after a catalytic reaction with the gas sample, through which a gas sample flows.
  • a light guide member that forms a light guide path along the one axis, and a detection unit that detects the fluorescence that has passed through the light guide path.
  • FIG. 1 is a cross-sectional view illustrating a configuration of a detection device according to Example 1.
  • FIG. It is an expanded sectional view of the reaction part of FIG.
  • FIG. 6 is an explanatory diagram illustrating an optical path of excitation light of the detection apparatus according to the first embodiment.
  • FIG. 3 is an explanatory diagram for explaining an optical path of fluorescence of the detection apparatus according to the first embodiment.
  • 6 is a cross-sectional view illustrating a configuration of a detection device according to Example 2.
  • FIG. FIG. 6 is an explanatory diagram illustrating an optical path of excitation light of a detection device according to Example 2.
  • FIG. 10 is a cross-sectional view illustrating a configuration of a detection device according to a modification example of Example 2.
  • FIG. 6 is a cross-sectional view illustrating a configuration of a detection device according to Embodiment 3.
  • FIG. FIG. 6 is a cross-sectional view illustrating a configuration of a detection device according to Example 4.
  • FIG. 10 is an explanatory diagram illustrating an optical path of excitation light of a detection device according to Example 4.
  • FIG. 10 is an explanatory diagram for explaining an optical path of fluorescence of a detection apparatus according to Example 4.
  • 10 is a cross-sectional view illustrating a configuration of a detection device according to Embodiment 5.
  • FIG. FIG. 10 is a cross-sectional view illustrating a configuration of a detection device according to Example 6.
  • FIG. 1 shows a cross section along one axis AX of a biosensor 10 as a detection apparatus according to an embodiment of the present invention.
  • a biosensor 10 as a detection device is a device that detects fluorescence emitted by a coenzyme that binds to an apoenzyme and detects a substrate that is a detection target.
  • the coenzyme used for detection of the substrate of the biosensor 10 is excited by excitation light in one state before and after the reaction of the substrate and emits fluorescence. Therefore, the biosensor 10 detects the substrate by utilizing the change in the amount of fluorescence emitted by the coenzyme due to the reaction of the substrate.
  • NADH reduced nicotinamide adenine dinucleotide
  • S-ADH catalyzes the reaction in which the substrate acetone is reduced to 2-propanol.
  • NADH which is a coenzyme is oxidized to NAD + (oxidized nicotinamide adenine dinucleotide) by an enzymatic reaction.
  • NADH emits fluorescence upon receiving excitation light of a predetermined wavelength, but does not emit fluorescence even when NAD + receives excitation light of the same wavelength. Therefore, the fluorescence intensity detected before and after this reaction varies.
  • the biosensor 10 of the present invention is a device that measures the concentration of a substrate by measuring the amount of fluorescence emitted from the NADH.
  • a light source LT is a light emitting device that emits excitation light.
  • the light source LT is, for example, an ultraviolet light emitting diode that emits ultraviolet light having a peak wavelength of 340 nm as excitation light.
  • the light emitting device is not limited to the ultraviolet light emitting diode, and for example, an ultraviolet laser diode, a mercury lamp, or the like can be used.
  • an excitation light optical system 20 that is an optical system for the excitation light emitted from the light source LT is provided.
  • the excitation light optical system 20 condenses the excitation light toward one axis AX.
  • One axis AX is the same axis as the optical axis of the excitation light in this embodiment.
  • the excitation light optical system 20 includes a collimator lens 21 that converts the excitation light into parallel light, and a ball lens 22 that is a condenser lens that condenses the excitation light that has been converted into parallel light by the collimator lens 21 onto one axis AX. including.
  • the excitation light optical system 20 is configured to have at least a numerical aperture higher than that of the optical fiber.
  • the focal length of the ball lens 22 is short among the condenser lenses, the configuration of the biosensor 10 can be further reduced. Further, the ball lens 22 has a large numerical aperture (NA) among the condensing lenses, and can take in more excitation light.
  • NA numerical aperture
  • an excitation light bandpass filter EF that transmits the wavelength of the excitation light.
  • the band transmitted by the excitation light bandpass filter EF is a band including the wavelength of excitation light excited by the coenzyme.
  • NADH is used as a coenzyme. NADH absorbs ultraviolet rays of 340 nm and emits fluorescence. Accordingly, the range of wavelengths transmitted by the excitation light bandpass filter EF is 330 to 350 nm.
  • a flow cell 30 is provided on one on-axis AX.
  • the flow cell 30 functions as a reaction unit in which the enzyme reaction shown in Chemical Formula 1 is performed.
  • the flow cell 30 includes a gas channel 31 through which a gas sample containing a substrate flows, a solution channel 32 as a solution holding unit that holds a solution containing a coenzyme, and an enzyme holding film 33 that holds an enzyme.
  • the solution flow path 32 may have a structure such as a tube through which a solution containing a coenzyme flows, or may have a structure such as a sealed container that does not flow a solution. Good.
  • the substrate contains either a ketone group or an aldehyde group.
  • a coenzyme that emits fluorescence when excited by excitation light in one state before and after the reaction of the substrate is used. Examples of such coenzymes include NADH and NADPH (reduced nicotinamide adenine dinucleotide phosphate).
  • NADH and NADPH reduced nicotinamide adenine dinucleotide phosphate
  • NADH or NADPH is used as a coenzyme, for example, alanine dehydrogenase, alcohol dehydrogenase, aldehyde dehydrogenase, isocitrate dehydrogenase, uridine-5′-diphospho-glucose dehydrogenase, galactose dehydrase
  • alanine dehydrogenase for example, alanine dehydrogenase, alcohol dehydrogenase, aldehyde dehydrogenase, isocitrate dehydrogenase, uridine-5′-diphospho-glucose dehydrogenase, galactose dehydrase
  • Elementary enzyme formate dehydrogenase, glyceraldehyde-3-phosphate dehydrogenase, glycerol dehydrogenase, glycerol-3-phosphate dehydrogenase, glucose dehydrogenase, glucose-6-
  • the light guide member 40 is provided in contact with the flow cell 30 on one axis AX.
  • the light guide member 40 is formed in a cylindrical shape in the present embodiment.
  • the light guide member 40 may have a shape other than a cylindrical shape, and may be, for example, a cylindrical shape having a non-planar end surface, a polygonal column shape, or a truncated cone shape.
  • the light guide member 40 is made of the same material such as glass having a uniform refractive index. Note that the light guide member 40 is not limited to the same material such as glass having a uniform refractive index, and may be configured of, for example, two materials of a core and a clad having different refractive indexes. Further, the light guide member 40 may be made of a material that has little absorption with respect to the fluorescence wavelength to be measured, for example, an absorption coefficient of 0.1 or less.
  • the light guide member 40 has a light guide path 41 formed along one axis AX.
  • a fluorescence optical system 50 that is an optical system for fluorescence emitted from the light guide member 40 is provided.
  • the fluorescence optical system 50 condenses the fluorescence emitted from the light guide member 40 toward one axis AX.
  • the fluorescent optical system 50 includes a collimating lens 51 that converts the fluorescent light into parallel light, and a condensing lens 52 that condenses the fluorescent light converted into parallel light by the collimating lens 51 on one axis AX.
  • a fluorescent bandpass filter FF that transmits a band including the wavelength of fluorescence.
  • the wavelength of fluorescence emitted by excitation of NADH as a coenzyme is 450 to 510 nm, more specifically, around 491 nm. Therefore, in this embodiment, the wavelength range transmitted by the fluorescent bandpass filter FF is 440 to 510 nm.
  • a detection unit 60 that detects fluorescence that has passed through the fluorescence optical system 50 is provided.
  • the detection unit 60 includes a photomultiplier tube, a photodiode detector, and a spectrophotometer including these, and detects the concentration of the substrate in the gas sample based on the detected fluorescence light quantity or spectral characteristics.
  • Case C is formed in a cylindrical shape covering the periphery of the light source LT, the excitation light optical system, the flow cell 30, the light guide member 40, the fluorescence optical system, and the detection unit 60. That is, the case C accommodates each of the light source LT, the excitation light optical system 20, the flow cell 30, the light guide member 40, the fluorescence optical system 50, and the detection unit 60 therein. Accordingly, the case C is configured so that outside light does not enter the case C.
  • the case C has two through holes HA provided through the case C in a direction perpendicular to the one axis AX.
  • the gas flow path 31 can be mounted on one axis AX. That is, the two through holes HA function as a first mounting portion that can mount the gas flow path 31 on one axis AX.
  • the case C is formed with two through holes HB provided through the case C in a direction perpendicular to the one axis AX.
  • the solution flow path 32 having a tube structure By inserting the solution flow path 32 having a tube structure into the two through holes HB, the solution flow path 32 can be mounted on one axis AX. That is, the two through holes HB function as a second mounting portion that can mount the solution flow path 32 on one axis AX.
  • the case C is formed with a protruding portion P formed so as to protrude so that inner walls facing each other approach each other in a direction perpendicular to the one axis AX.
  • the protrusion P is formed along the circumferential direction of the inner wall of the case C. Further, the protruding portion P is formed between the through hole HA and the through hole HB on one axis AX.
  • the enzyme holding film 33 is mounted on one axis AX by fitting the enzyme holding film 33 into the protruding portion P. In other words, the protruding portion P functions as a third mounting portion that can mount the enzyme holding film 33 on one axis AX.
  • the gas flow path 31, the liquid flow path 32, and the enzyme holding film 33 can be detached from the case C, respectively.
  • at least one of the gas channel 31, the liquid channel 32, and the enzyme holding film 33 may be detachable, and the rest may be fixed to the case C.
  • the through-hole HB does not need to be provided.
  • the groove G may be formed along the circumferential direction of the inner wall of the case C.
  • FIG. 2 shows an enlarged cross section of the flow cell 30 along one axis AX.
  • a gas flow path 31 that has a window W that transmits excitation light and through which a gas sample containing a substrate flows.
  • a through hole H ⁇ b> 1 that penetrates the gas flow path 31 and the outside is provided on the detection section 60 side of the gas flow path 31.
  • a solution channel 32 through which a solution containing a coenzyme flows is provided on the detection unit 60 side of the flow cell 30.
  • the solution flow path 32 includes an upstream connection portion provided on the upstream side in the solution flow direction, a downstream connection portion provided on the downstream side in the solution flow direction, an upstream connection portion, and a downstream connection. And a curved portion that is curved toward the light source LT side.
  • a through hole H2 that penetrates the solution channel 32 and the outside is provided.
  • the solution flowing through the solution flow path 32 contains a coenzyme and a buffer solution having a pH value considering the optimum pH value of the enzyme or coenzyme as components.
  • the enzyme holding film 33 for holding the enzyme is provided in contact with both the gas channel 31 and the solution channel 32 so as to block the through hole H1 of the gas channel 31 and the through hole H2 of the solution channel 32. ing. That is, the enzyme holding film 33 is a diaphragm that allows the held enzyme to contact the solution in the solution channel 32 and the gas sample in the gas channel 31 and separates the solution channel 32 and the gas channel 31. .
  • the enzyme holding film 33 is obtained by immobilizing an enzyme on a carrier that is a film material.
  • the carrier for the enzyme holding film 33 include polytetrafluoroethylene, polydimethylsiloxane, polypropylene, polyethylene, polymethyl methacrylate, polystyrene, polyvinylidene fluoride, nitrocellulose, and cellulose.
  • the flow cell 30 is formed to be recessed along one axis AX so as to go from the detection unit 60 side to the light source LT side, and has a through hole H3 penetrating the solution flow path 32 and the outside.
  • the through hole H ⁇ b> 3 includes a small diameter portion having a size equivalent to the outer diameter of the light guide member 40, and a large diameter portion formed by expanding from the small diameter portion toward the fluorescence optical system 50.
  • the light guide member 40 is held by the flow cell 30 by fitting the light guide member 40 to the small diameter portion.
  • the flow cell 30 functions as a holding member that holds the light guide member 40.
  • the flow cell 30 has a space SP between a side surface SS of the light guide member 40 extending along one axis AX and a wall portion of the enlarged diameter portion of the through hole H3.
  • the numerical aperture (NA) is given by the following equation.
  • NA numerical aperture
  • the light guide path 41 of the light guide member 40 may be formed so as to reduce the amount of excitation light guided. Specifically, the incident angle with respect to the light guide member 40 of at least a part of the excitation light that has passed through the solution flow path 32 of the flow cell 30 is greater than the maximum light reception angle that can be totally reflected by the inner surface of the light guide path 41 of the light guide member 40. It is better to make it larger.
  • FIG. 3 shows an aspect of the excitation light emitted from the light source LT.
  • the alternate long and short dash line arrow indicates the excitation light LT1.
  • the excitation light LT1 emitted from the light source LT is converted into parallel light by the collimator lens 21.
  • the excitation light LT1 that has been converted into parallel light by the collimator lens 21 is subjected to removal of light having a wavelength other than a predetermined band in the excitation light bandpass filter EF.
  • the excitation light LT1 that has passed through the excitation light bandpass filter EF is collected by the ball lens 22 toward the solution flow path 32 of the flow cell 30.
  • the ball lens 22 has a short focal length even among the biconvex lenses. Therefore, by using the ball lens 22 in the excitation light optical system 20, it is possible to increase the amount of excitation light LT1 incident at an incident angle larger than the maximum light receiving angle of the light guide path 41.
  • the ball lens 22 has a low aberration but has a short focal length, which is advantageous for downsizing the biosensor 10. For this reason, by increasing the diameter of the light guide member 40, defocus due to the deterioration of the aberration of the ball lens 22 is allowed. That is, the diameter of the light guide member 40 is ideally the minimum diameter that allows the size of the light source LT and lens aberration.
  • the excitation light LT1 is an annular light and the diameter of the annular light incident on the ball lens 22 is increased, the aberration of the ball lens 22 can be reduced and the focal length can be further shortened. For this reason, it becomes easy to increase the amount of the excitation light LT1 incident beyond the maximum light receiving angle of the light guide path 41.
  • the excitation light optical system 20 including the ball lens 22 is configured with a numerical aperture larger than the numerical aperture of the light guide member 40. For this reason, the excitation light LT1 incident on the light guide path 41 at an acute angle with respect to the one axis AX increases. That is, the amount of excitation light LT1 incident on the light guide 41 at an incident angle larger than the maximum light receiving angle of the light guide 41 is increased. As a result, the amount of the excitation light LT1 that is transmitted outside without being guided through the light guide member 40 increases.
  • the excitation light LT1 exhibits an annular distribution even when the optical system is not configured with an optical system larger than the numerical aperture of the light guide member 40, as described below, Collimation of the excitation light LT1 (light guide to the detection unit 60) can be suppressed by the arrangement of the subsequent collimating lens.
  • the excitation light LT1 that has passed through the flow cell 30 enters the light guide member 40 at various incident angles.
  • the excitation light LT1 that is incident at an incident angle that is less than the maximum light reception angle that can be totally reflected by the inner surface of the light guide 41 has a certain distribution due to the influence of the light source LT and the excitation light optical system 20.
  • the distribution of the excitation light LT1 is also maintained in the light guide path 41.
  • the density of the excitation light LT1 is generated in the light guide path 41.
  • the collimating lens 51 is arranged so that the lightest light of the excitation light LT1 is collimated by the collimating lens 51. That is, the collimating lens 51 is arranged so that the excitation light LT1 is defocused at the focal position of the collimating lens 51 in the light guide path 41. By arranging the collimating lens 51 in this way, a lot of excitation light L1 can be diffused without being collimated by the collimating lens 51.
  • the excitation light LT1 converted into parallel light by the collimating lens 51 is reflected by the fluorescent bandpass filter FF.
  • FIG. 4 shows a mode of fluorescence emitted from the flow cell 30.
  • the alternate long and short dash line indicates the fluorescence LT2.
  • the coenzyme receives the excitation light LT1, it emits fluorescence LT2.
  • the fluorescence LT2 passes through the solution in the solution flow path 32 and enters the light guide path 41 of the light guide member 40.
  • the fluorescent light LT 2 guided through the light guide path 41 is emitted from the emission end of the light guide member 40 toward the collimator lens 51.
  • Fluorescence LT2 collimated by the collimating lens 51 removes light having a wavelength other than a predetermined band by the fluorescence bandpass filter FF.
  • the fluorescence LT2 that has passed through the fluorescence bandpass filter FF is condensed toward the detection unit 60 by the condenser lens.
  • the excitation light LT1 emitted from the light source LT is irradiated to the flow cell 30 without passing through the optical fiber used in the conventional detection device.
  • the biosensor 10 has high utilization efficiency of the excitation light LT1, and can increase the detection accuracy of the specific substance by increasing the amount of fluorescence emitted from the coenzyme. Further, since the biosensor 10 does not have an optical fiber, the number of parts can be reduced, and the apparatus can be downsized.
  • the biosensor 10 also has a light guide member 40 provided in contact with the flow cell 30. Thereby, a part of the excitation light LT1 that has entered the light guide 41 beyond the maximum light receiving angle of the light guide 41 passes through the light guide 41 without being guided. Therefore, the amount of excitation light LT1 detected by the detection unit 60 can be reduced, and detection accuracy can be improved.
  • the biosensor 10 according to Example 2 will be described.
  • the biosensor 10 according to the second embodiment is different from the biosensor 10 according to the first embodiment in that the biosensor 10 includes a light shielding member for shaping the radiation distribution of the excitation light LT1 emitted from the light source LT into an annular shape.
  • the biosensor 10 includes a light shielding member for shaping the radiation distribution of the excitation light LT1 emitted from the light source LT into an annular shape.
  • symbol to the same location and it is the same also about subsequent Examples.
  • FIG. 5 shows a cross section along one axis AX of the biosensor 10 according to the second embodiment.
  • the excitation light optical system 20 includes a light shielding member 70 that is arranged on one axis AX and that can shield the excitation light LT1.
  • the light shielding member 70 is formed in a disk shape, for example.
  • the size of the light shielding member 70 may be formed larger than the diameter of the light guide path 41 of the light guide member 40.
  • FIG. 6 shows an aspect of the excitation light LT1 emitted from the light source LT in the biosensor 10 of the second embodiment.
  • the one-dot chain line arrow indicates the excitation light LT1.
  • a lot of excitation light LT1 is incident on the light guide path 41 at an angle larger than the total reflection angle. Thereby, most of the excitation light LT1 passes through the light guide member 40 without being guided through the light guide path 41.
  • the excitation light LT1 that has not been absorbed by the coenzyme (NADH) in the solution flow path 32 enters the light guide member 40.
  • a part of the excitation light LT1 is incident at a wide angle with respect to the axis AX, that is, at an incident angle larger than the maximum light receiving angle that can be totally reflected by the inner surface of the light guide path 41 of the light guide member 40.
  • the excitation light LT1 incident at an incident angle larger than the maximum light receiving angle is transmitted through the light guide 41 from the side surface SS to the outside of the light guide member 40.
  • the excitation light LT1 that travels straight on one axis AX can be blocked. Further, the incident angle of the excitation light LT1 incident on the light guide member 40 can be increased, and a large amount of the excitation light LT1 can be prevented from being guided in the light guide path 41. As a result, the amount of excitation light LT1 detected by the detection unit 60 can be reduced, and the detection accuracy can be improved.
  • the excitation light optical system 20 includes the light shielding member 70 as in the present embodiment, the amount of excitation light LT1 that guides the light guide path 41 can be reduced. Therefore, the biosensor 10 may be configured without providing the fluorescence optical system 50.
  • FIG. 7 shows a configuration of a modification of the biosensor 10 according to the present embodiment.
  • the biosensor 10 does not have the fluorescence optical system 50 and the fluorescence filter FF.
  • the biosensor 10 it is possible to reduce the size of the biosensor 10.
  • the biosensor 10 according to Example 3 will be described.
  • the biosensor 10 according to the third embodiment is different from the biosensor 10 according to the first and second embodiments in that the shape of the flow cell 30 is different.
  • FIG. 8 shows an enlarged cross section of the flow cell 30 along one axis AX of the biosensor 10 according to the third embodiment.
  • the light guide member 40 is formed such that a portion 34 in contact with the solution flow path 32 of the flow cell 30 is narrowed toward the fluorescence optical system 50. That is, the portion 34 of the light guide member 40 that contacts the solution flow path 32 of the flow cell 30 is inclined so as to have an angle with respect to one axis AX. Therefore, the excitation light LT1 applied to the portion 34 of the light guide member 40 that contacts the solution flow path 32 of the flow cell 30 is reflected toward the solution flow path 32 of the flow cell 30.
  • a part of the excitation light LT1 incident on the light guide member 40 can be reflected toward the solution flow path 32 of the flow cell 30, so that the fluorescence The light emission efficiency of LT2 can be improved.
  • a portion 34 that contacts the solution flow path 32 of the flow cell 30 may be provided with a reflection member that reflects the excitation light LT1. Further, in order to diffusely reflect the excitation light LT1, the portion of the flow cell 30 that contacts the solution flow path 32 may have an uneven surface.
  • the biosensor 10 according to Example 4 will be described.
  • the biosensor 10 according to the fourth embodiment is different from the biosensor 10 according to the first embodiment in that it does not include the excitation light optical system 20.
  • FIG. 9 shows a cross section along one axis AX of the biosensor 10 according to the fourth embodiment.
  • a long pass filter LF for cutting a band including the wavelength of the excitation light LT1 is provided between the collimating lens 51 and the fluorescent band pass filter FF.
  • FIG. 10 shows an aspect of the excitation light LT1 emitted from the light source LT of the biosensor 10 according to the fourth embodiment.
  • the alternate long and short dash line arrow indicates the excitation light LT1.
  • the excitation light LT ⁇ b> 1 emitted from the light source LT passes through the flow cell 30 and is incident on the light guide member 40.
  • the excitation light LT1 exceeding the maximum light receiving angle of the light guide 41 passes through the light guide 41 without being guided.
  • the excitation light LT1 guided through the light guide path 41 is collimated by the collimating lens 51 and attenuated by the long pass filter LF.
  • FIG. 11 shows an aspect of the fluorescence LT2 emitted from the flow cell 30 of the biosensor 10 according to the fourth embodiment.
  • the alternate long and short dash line arrow indicates the fluorescence LT2.
  • the fluorescence LT2 emitted in the solution flow path 32 of the flow cell 30 is guided in the light guide path 41 of the light guide member 40.
  • the fluorescence LT2 emitted from the light guide member 40 is collimated by the collimating lens 51, and passes through the long pass filter LF and the fluorescence band pass filter FF.
  • the fluorescence LT2 that has passed through the fluorescence bandpass filter FF is condensed toward the detection unit 60 through the condenser lens 52.
  • the excitation light optical system 20 since the excitation light optical system 20 is not provided, it is possible to directly irradiate the solution flow path 32 with high intensity excitation light. . For this reason, the light emission amount of the fluorescence LT2 can be increased, and the size of the device can be reduced by reducing the number of parts of the device.
  • a biosensor 10 according to Example 5 will be described.
  • the biosensor 10 according to the fifth embodiment is different from the biosensor 10 according to the first to fourth embodiments in that the shape of the gas flow path 31 of the flow cell 30 is different.
  • FIG. 12 shows a cross section along one axis AX of the biosensor 10 according to the fifth embodiment.
  • the excitation light optical system 20 has a collimating lens 21, but does not have a ball lens 22.
  • the gas flow path 31 of the flow cell 30 has a lens portion 31 a formed so as to have a curved surface that is convex toward the enzyme holding film 33 around the one axis AX.
  • the lens unit 31 a condenses the excitation light LT ⁇ b> 1 converted into parallel light by the collimating lens 21 toward the enzyme holding film 33. Therefore, according to the biosensor 10 according to the present embodiment, the ball lens 22 of the excitation light optical system 20 is not necessary. As a result, the number of parts of the apparatus is reduced, and the apparatus can be miniaturized.
  • a biosensor 10 according to Example 6 will be described.
  • the biosensor 10 according to the sixth embodiment is different from the biosensor 10 according to the first to fifth embodiments in that the arrangement positions of the light source LT and the detection unit 60 are different.
  • the light source LT, the excitation light optical system 20, the flow cell 30, the light guide member 40, the fluorescence optical system 50, and the detection unit 60 are arranged on one axis AX, but the light source LT In addition, at least one of the detection units 60 may not be arranged on one axis AX.
  • FIG. 13 shows a cross section along one axis AX of the biosensor 10 according to the sixth embodiment.
  • the light source LT and the detection unit 60 are respectively disposed on an axis AX2 and an axis AX3 that are orthogonal to one axis AX.
  • the mirror MR1 and the mirror MR2 are disposed at a position where the axis AX2 and the axis AX3 intersect with one axis AX. That is, the excitation light LT1 emitted from the light source LT is reflected by the mirror MR1 so as to reach the excitation light optical system 20.
  • the fluorescence LT2 that has passed through the fluorescence optical system 50 is reflected by the mirror MR2 so as to reach the detection unit 60.
  • the excitation light optical system 20 and the fluorescence optical system 50 are arranged on one axis AX that is the same axis as the optical axis of the excitation light LT1.
  • the excitation light optical system 20 and the fluorescence optical system 50 do not have to be arranged on one axis AX that is the same as the optical axis of the excitation light LT1, and the excitation light
  • the optical axis of LT1 and the optical axis of fluorescence LT2 may deviate from the axis AX as long as the fluorescence LT2 can reach the detection unit 60.

Landscapes

  • Health & Medical Sciences (AREA)
  • Nuclear Medicine, Radiotherapy & Molecular Imaging (AREA)
  • Physics & Mathematics (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Analytical Chemistry (AREA)
  • Biochemistry (AREA)
  • General Health & Medical Sciences (AREA)
  • General Physics & Mathematics (AREA)
  • Immunology (AREA)
  • Pathology (AREA)
  • Investigating, Analyzing Materials By Fluorescence Or Luminescence (AREA)

Abstract

L'invention concerne un dispositif de détection qui peut améliorer la précision de détection d'une substance spécifique grâce à l'amélioration de l'efficacité d'utilisation de la lumière d'excitation et de la lumière fluorescente et qui peut réaliser une miniaturisation de dispositif. Ce dispositif de détection comprend : une partie de réaction qui est disposée sur un axe et qui comprend un trajet d'écoulement de solution à travers lequel une solution contenant une coenzyme excitée par une lumière d'excitation pour émettre de la lumière fluorescente s'écoule, un trajet d'écoulement de gaz à travers lequel s'écoule un échantillon de gaz, et un film de maintien d'oxygène qui contient de l'oxygène pour catalyser la réaction de l'échantillon de gaz avec la coenzyme ; un élément de guide d'ondes qui est disposé en contact avec la partie de réaction sur l'axe et qui forme un guide d'ondes le long de l'axe ; et une partie de détection qui est disposée sur l'axe et qui détecte la lumière fluorescente qui a traversé le guide d'ondes.
PCT/JP2019/010348 2018-03-29 2019-03-13 Dispositif de détection WO2019188304A1 (fr)

Priority Applications (1)

Application Number Priority Date Filing Date Title
JP2020509875A JP6992164B2 (ja) 2018-03-29 2019-03-13 検出装置

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
JP2018064398 2018-03-29
JP2018-064398 2018-03-29

Publications (1)

Publication Number Publication Date
WO2019188304A1 true WO2019188304A1 (fr) 2019-10-03

Family

ID=68061702

Family Applications (1)

Application Number Title Priority Date Filing Date
PCT/JP2019/010348 WO2019188304A1 (fr) 2018-03-29 2019-03-13 Dispositif de détection

Country Status (2)

Country Link
JP (1) JP6992164B2 (fr)
WO (1) WO2019188304A1 (fr)

Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN111307769A (zh) * 2019-12-11 2020-06-19 长江大学 一种基于指示剂型荧光染料的酶反应检测装置
JP2021153451A (ja) * 2020-03-26 2021-10-07 パイオニア株式会社 検出装置
WO2022266098A1 (fr) * 2021-06-14 2022-12-22 Si-Ware Systems Analyseur de fluide optique
US12031904B2 (en) 2021-06-14 2024-07-09 Si-Ware Systems Optical fluid analyzer
WO2024185521A1 (fr) * 2023-03-03 2024-09-12 株式会社ヘルスケアビジョン Appareil de mesure non invasif

Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20080123095A1 (en) * 2004-07-26 2008-05-29 Danmarks Tekniske Universitet On-Chip Spectroscopy
JP2013033008A (ja) * 2011-08-03 2013-02-14 Sony Corp 光学分析装置及び光学分析方法
WO2013031896A1 (fr) * 2011-09-01 2013-03-07 三菱重工業株式会社 Mécanisme d'analyse d'une composition fluidique, dispositif de mesure de la quantité de chaleur générée et centrale électrique, et procédé d'analyse d'une composition liquide
JP2016509206A (ja) * 2012-12-21 2016-03-24 マイクロニクス, インコーポレイテッド 携帯型蛍光検出システムおよびマイクロアッセイカートリッジ
JP2016220573A (ja) * 2015-05-28 2016-12-28 国立大学法人 東京医科歯科大学 Uv−led光源を用いたバイオセンサシステム

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20080123095A1 (en) * 2004-07-26 2008-05-29 Danmarks Tekniske Universitet On-Chip Spectroscopy
JP2013033008A (ja) * 2011-08-03 2013-02-14 Sony Corp 光学分析装置及び光学分析方法
WO2013031896A1 (fr) * 2011-09-01 2013-03-07 三菱重工業株式会社 Mécanisme d'analyse d'une composition fluidique, dispositif de mesure de la quantité de chaleur générée et centrale électrique, et procédé d'analyse d'une composition liquide
JP2016509206A (ja) * 2012-12-21 2016-03-24 マイクロニクス, インコーポレイテッド 携帯型蛍光検出システムおよびマイクロアッセイカートリッジ
JP2016220573A (ja) * 2015-05-28 2016-12-28 国立大学法人 東京医科歯科大学 Uv−led光源を用いたバイオセンサシステム

Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN111307769A (zh) * 2019-12-11 2020-06-19 长江大学 一种基于指示剂型荧光染料的酶反应检测装置
JP2021153451A (ja) * 2020-03-26 2021-10-07 パイオニア株式会社 検出装置
WO2022266098A1 (fr) * 2021-06-14 2022-12-22 Si-Ware Systems Analyseur de fluide optique
US12031904B2 (en) 2021-06-14 2024-07-09 Si-Ware Systems Optical fluid analyzer
WO2024185521A1 (fr) * 2023-03-03 2024-09-12 株式会社ヘルスケアビジョン Appareil de mesure non invasif

Also Published As

Publication number Publication date
JPWO2019188304A1 (ja) 2021-02-25
JP6992164B2 (ja) 2022-01-13

Similar Documents

Publication Publication Date Title
WO2019188304A1 (fr) Dispositif de détection
US6710870B1 (en) Method and device for measuring luminescence
US7801394B2 (en) Sensitive emission light gathering and detection system
CN110621980B (zh) 气体测量系统
US5221958A (en) Reflection fluorometer
US7405824B2 (en) Optical coupling system of light measuring device and sample
JP2010243270A (ja) 複合型マルチパスセルおよびガス測定器
JP2009156659A (ja) 測定装置及び測定方法
JP7042047B2 (ja) 検出装置
JP3754440B2 (ja) 自動化されたシステム、及びサンプルの分析方法
JP2021153451A (ja) 検出装置
EP2565629B1 (fr) Analyseur automatique
JP7128007B2 (ja) 気体成分検出用フローセル及び検出装置
JP2020171239A (ja) 気体成分検出用フローセル及び気体成分検出装置
JP2021193967A (ja) 交換部品
US7012692B2 (en) Photothermal conversion spectroscopic analysis method, and photothermal conversion spectroscopic analysis apparatus for carrying out the method
US20070190642A1 (en) Concentrators for Luminescent Emission
JP2020171240A (ja) 気体成分検出用フローセル及び気体成分検出装置
JP5800472B2 (ja) 光源装置
JP2003344323A (ja) 光熱変換分光分析方法およびその方法を実行する光熱変換分光分析装置
JP2003149154A (ja) 分光蛍光光度計
WO2022168374A1 (fr) Système optique d'émission, dispositif d'émission et dispositif de mesure optique
JP2006242623A (ja) フローサイトメータ及び蛍光集光方法
CN218445140U (zh) 原子荧光光度计
JP3016640B2 (ja) 光導波路型バイオセンサ

Legal Events

Date Code Title Description
121 Ep: the epo has been informed by wipo that ep was designated in this application

Ref document number: 19778124

Country of ref document: EP

Kind code of ref document: A1

ENP Entry into the national phase

Ref document number: 2020509875

Country of ref document: JP

Kind code of ref document: A

NENP Non-entry into the national phase

Ref country code: DE

122 Ep: pct application non-entry in european phase

Ref document number: 19778124

Country of ref document: EP

Kind code of ref document: A1