WO2020073867A1 - 生物芯片及其制造方法、操作方法、生物检测系统 - Google Patents
生物芯片及其制造方法、操作方法、生物检测系统 Download PDFInfo
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- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- 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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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L3/00—Containers or dishes for laboratory use, e.g. laboratory glassware; Droppers
- B01L3/50—Containers for the purpose of retaining a material to be analysed, e.g. test tubes
- B01L3/502—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures
- B01L3/5027—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip
- B01L3/502761—Containers for the purpose of retaining a material to be analysed, e.g. test tubes with fluid transport, e.g. in multi-compartment structures by integrated microfluidic structures, i.e. dimensions of channels and chambers are such that surface tension forces are important, e.g. lab-on-a-chip specially adapted for handling suspended solids or molecules independently from the bulk fluid flow, e.g. for trapping or sorting beads, for physically stretching molecules
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- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Q—MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6869—Methods for sequencing
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- B01L2200/00—Solutions for specific problems relating to chemical or physical laboratory apparatus
- B01L2200/06—Fluid handling related problems
- B01L2200/0647—Handling flowable solids, e.g. microscopic beads, cells, particles
- B01L2200/0668—Trapping microscopic beads
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- B01L2200/00—Solutions for specific problems relating to chemical or physical laboratory apparatus
- B01L2200/12—Specific details about manufacturing devices
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- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2300/00—Additional constructional details
- B01L2300/06—Auxiliary integrated devices, integrated components
- B01L2300/0627—Sensor or part of a sensor is integrated
- B01L2300/0645—Electrodes
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2300/00—Additional constructional details
- B01L2300/08—Geometry, shape and general structure
- B01L2300/0809—Geometry, shape and general structure rectangular shaped
- B01L2300/0819—Microarrays; Biochips
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2300/00—Additional constructional details
- B01L2300/08—Geometry, shape and general structure
- B01L2300/0887—Laminated structure
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2300/00—Additional constructional details
- B01L2300/12—Specific details about materials
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- B—PERFORMING OPERATIONS; TRANSPORTING
- B01—PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
- B01L—CHEMICAL OR PHYSICAL LABORATORY APPARATUS FOR GENERAL USE
- B01L2400/00—Moving or stopping fluids
- B01L2400/04—Moving fluids with specific forces or mechanical means
- B01L2400/0403—Moving fluids with specific forces or mechanical means specific forces
- B01L2400/0415—Moving fluids with specific forces or mechanical means specific forces electrical forces, e.g. electrokinetic
Definitions
- the embodiments of the present disclosure relate to a biochip, its manufacturing method, operation method, and biological detection system.
- Gene chip technology refers to the use of microarray technology to attach high-density gene (DNA) fragments to a solid surface such as glass slides in a certain order or arrangement in a certain way, and fluorescently labeled DNA probes through alkali Based on the principle of complementary hybridization, it is a technique for a large number of gene expression and monitoring research.
- DNA high-density gene
- At least one embodiment of the present disclosure provides a biochip, including: a base substrate; a plurality of working units disposed on the base substrate; wherein, each of the working units includes a working element configured to contact the target substance
- the working element includes a metal electrode and an electric field controllable surface modification layer on the surface of the metal electrode that is remote from the base substrate and facing the target substance.
- the electric field controllable surface modification layer includes an electric field controllable isomerized organic molecule, and an end of the electric field controllable isomerized organic molecule is connected to the The surface of the metal electrode.
- the organic molecule with controlled electric field isomerization includes thioalcoholic acid or thioalcoholic acid derivative molecules, the thioalcoholic acid or the thioxo
- the alkyd derivative molecule is connected to the surface of the metal electrode through a mercapto group at the end.
- the material of the metal electrode includes at least one of gold and silver.
- the biochip provided in at least one embodiment of the present disclosure further includes a flow channel defining layer provided on the base substrate, wherein the flow channel defining layer includes a flow channel, and the fluid of the target substance passes through the The flow channel reaches at least one of the plurality of work units.
- the flow channel includes oppositely disposed side walls, and the oppositely disposed side walls form a plurality of branches, and the plurality of branches form a cross and cross Connected at the intersection.
- each of the working units further includes a switching element, the switching element includes a control terminal, a first end, and a second end, the working element and the switch The second end of the element is electrically connected, and the switching element is configured to determine whether to apply an operating voltage to the working element according to a control signal.
- the base substrate is a glass substrate.
- the target substance includes a gene fragment, and the gene fragment is fixed on the working element.
- the end groups of the gene fragments include mercapto groups, amino groups, hydroxyl groups, carboxyl groups, phosphate groups, alkoxy groups, amine groups, fluorine-containing groups, and quaternary amino groups. And one or more of quaternary phosphorus base.
- the biochip provided in at least one embodiment of the present disclosure further includes a counter substrate, wherein the counter substrate is disposed opposite to the base substrate, and the working unit is located on the counter substrate and the base substrate between.
- the opposing substrate includes an opposing base and an opposing electrode, and the opposing electrode is disposed on the opposing base opposite to the base substrate On the surface and opposite to the working unit.
- the biochip provided in at least one embodiment of the present disclosure further includes a flow channel defining layer disposed on the base substrate, wherein the flow channel defining layer includes a flow channel, and the flow channel includes oppositely disposed sides Wall, the side wall abuts against the opposite substrate.
- At least one embodiment of the present disclosure also provides a biological detection system, including a control unit and the biochip according to any embodiment of the present disclosure, wherein the control unit is configured to process the plurality of working units of the biochip Apply control signals.
- At least one embodiment of the present disclosure also provides a method for manufacturing a biochip, including: forming a plurality of working units on a base substrate, wherein each of the working units includes a working element for contacting with a target substance, the The working element includes a metal electrode and an electric field controllable surface modification layer formed on the surface of the metal electrode away from the base substrate and facing the target substance; applying control to a selected working unit among the plurality of working units Signal to form a control electric field by the working element of the selected working unit, the control electric field controlling the property of the electric field controllable surface modification layer of the working element of the selected working unit to control the Fluid operation.
- At least one embodiment of the present disclosure further provides an operation method of any of the above biochips, including: applying a control signal to a selected working unit among the plurality of working units, and forming a control by working elements of the selected working unit An electric field, the control electric field controls the properties of the electric field controllable surface modification layer of the working element of the selected working unit to control the operation of the fluid including the target substance.
- the controlled electric field causes the electric field controllable isomerized organic molecules in the electric field controllable surface modification layer to lie down on the surface of the metal electrode ,
- the electric field controllable surface modification layer exhibits hydrophobicity, when the target substance is located on the electric field controllable surface modification layer, the target substance is spaced from the metal electrode, and the target substance is in the electric field Controls the flow on the surface modification layer.
- the controlled electric field causes the electric field controllable isomerized organic molecules in the electric field controllable surface modification layer to stand on the surface of the metal electrode ,
- the electric field controllable surface modification layer exhibits hydrophilicity, when the target substance is located on the electric field controllable surface modification layer, the target substance contacts the metal electrode, and the target substance passes through the end Is connected to the surface of the metal electrode.
- FIG. 1 is a schematic block diagram of a biochip provided by an embodiment of the present disclosure
- FIG. 2 is a schematic diagram of flow channel distribution of a biochip provided by an embodiment of the present disclosure
- FIG. 3 is a schematic cross-sectional view of a biochip provided by an embodiment of the present disclosure.
- FIG. 5 is a schematic diagram of a target substance of a biochip provided by an embodiment of the present disclosure.
- 6A and 6B are schematic diagrams of a state of a controllable surface modification layer of an electric chip provided by an embodiment of the present disclosure
- FIG. 7 is a schematic flow diagram of a target substance of a biochip according to an embodiment of the present disclosure.
- FIG. 8 is a schematic diagram of a fixed position of a target substance of a biochip according to an embodiment of the present disclosure
- FIG. 9 is a schematic cross-sectional view of another biochip provided by an embodiment of the present disclosure.
- FIG. 10 is a schematic flow diagram of another biochip target substance provided by an embodiment of the present disclosure.
- FIG. 11 is a schematic block diagram of a biological detection system according to an embodiment of the present disclosure.
- FIG. 12 is a schematic flowchart of a method for manufacturing a biochip according to an embodiment of the present disclosure.
- Single nucleotide polymorphism (SNP) chip is a kind of gene chip.
- SNP chip is usually realized by combining microwell with microsphere structure, that is, the oligonucleotide and probe with address are passed through the amino group first. Connect to the glass microspheres, and then fill the microwells with glass microspheres containing different addresses.
- address refers to a sequence of oligonucleotides. Different sequences represent different addresses. Oligonucleotides are usually short-chain nucleotides including 20 or less bases.
- the distribution position of the microsphere structure of the SNP chip prepared in the above manner is difficult to control, that is, the distribution position of gene fragments (for example, probes) is difficult to control, and the distribution of gene fragments is highly random. Therefore, it is necessary to measure the oligonucleotide sequence as an address on each microsphere structure in advance to know the corresponding probe sequence on the microsphere structure. The distribution information of these probes needs to be provided to the user for later comparison when the chip is used for genetic testing, which increases labor cost and time cost.
- SNP chips are usually prepared based on microwell or nanowell technology, and silicon-based materials are mostly used, so the production cost of SNP chips is very high. The use of microsphere structure to graft oligonucleotide fragments also leads to increased production costs.
- At least one embodiment of the present disclosure provides a biochip, a method for manufacturing the same, an operation method, and a biodetection system.
- the biochip can realize the controllability of the fixed position of gene fragments, and can improve the fluorescent crosstalk between gene fragments. It is compatible with the semiconductor manufacturing process and the production cost is low, which helps to improve the detection accuracy and detection flux.
- At least one embodiment of the present disclosure provides a biochip including a base substrate and a plurality of working units.
- a plurality of working units are provided on the base substrate, and each of the working units includes a working element for contacting with a target substance, the working element includes a metal electrode and a substrate formed on the metal electrode away from the substrate The electric field on the surface of the substrate can control the surface modification layer.
- FIG. 1 is a schematic block diagram of a biochip provided by an embodiment of the present disclosure.
- the biochip 100 includes a base substrate 11 and a plurality of working units 12.
- a plurality of working units 12 are provided on the base substrate 11.
- Each working unit 12 includes a working element 121 for contact with the target substance.
- the working element 121 includes a metal electrode 1211 and an electric field controllable surface modification layer 1212 formed on the surface of the metal electrode 1211 away from the base substrate 11.
- the target substance is a gene fragment, and the gene fragment may include oligonucleotides, primers, probes, target DNA fragments or polypeptides, etc.
- the embodiments of the present disclosure do not limit this.
- different gene fragments may be fixed on different predetermined working elements 121 among the plurality of working elements 121, so that the fixed position of the gene fragments can be controlled.
- the biochip 100 to which the gene fragment is fixed can be used to detect the substance containing the gene to be detected separately, for example, by performing base complementary hybridization of the gene fragment fixed on the working element 121 and the gene to be detected, to detect the gene to be detected Perform testing, such as genetic sequencing.
- the biochip 100 can be applied to the field of biomolecule detection and other related fields.
- FIG. 2 is a schematic diagram of a flow channel distribution of a biochip provided by an embodiment of the disclosure
- FIG. 3 is a schematic cross-sectional diagram of a biochip provided by an embodiment of the disclosure.
- the biochip 200 includes a flow channel defining layer 13 disposed on a base substrate 11, and the flow channel defining layer 13 includes a flow channel 131, which may help to define the target substance Flow direction of the fluid on the base substrate 11, droplet size, etc.
- the plurality of working units 12 are distributed along the flow channel 131, for example, the plurality of working units 12 are uniformly distributed or non-uniformly distributed along the flow channel 131.
- the number of working units 12 in the biochip 200 is not limited, and may be 50,000 to 10,000,000, or may be other numbers, which is not limited by the embodiments of the present disclosure.
- multiple work units 12 are arranged in an array, including 100 rows and 100 columns, and the number is 10,000.
- the flow channel 131 is used to provide a flow channel for a fluid (eg, droplet) including the target substance, to allow the fluid including the target substance to flow through the flow channel 131 and reach at least one of the plurality of working units 12.
- a fluid eg, droplet
- the fixed position of the fragments can be controlled (how to drive the fluid to flow and how to fix the gene fragments will be described in detail later).
- the flow channel 131 includes multiple branches.
- a plurality of branches are crossed and connected at the intersection, and a plurality of working units 12 are distributed along the plurality of branches.
- the branches can be spread all over the base substrate 11 and the fluid including the target substance can reach any one of the working units 12 through the branches.
- the branches may be in any distribution manner, such as multiple concentric circles, multiple concentric rectangles, etc. The distribution manner of the branches may be determined according to actual needs.
- the working unit 12 is disposed on the base substrate 11 and is located in the flow channel 131.
- the working unit 12 includes a working element 121 and a switching element 122 that are electrically connected to each other.
- the working element 121 is disposed on the switching element 122.
- the working element 121 is located in and exposed to the flow path 131, whereby the working element 121 can It is in contact with the fluid flowing through the flow path 131.
- the base substrate 11 functions as support, protection, etc.
- the base substrate 11 may be a glass substrate, a plastic substrate, a quartz substrate, or a substrate made of other suitable materials, which is not limited by the embodiments of the present disclosure. Since the biochip 200 is compatible with a conventional semiconductor manufacturing process, the substrate made of the above materials can be used. Compared with a conventional biochip (such as an SNP chip) using a silicon-based substrate, the production cost can be effectively reduced.
- the switching element 122 is provided on the base substrate 11, and the switching element 122 is configured to determine whether to allow the operating voltage to be applied to the operating element 121 according to the control signal.
- the switching element 122 may be a three-terminal element such as a thin film transistor, and the switching element 122 includes a control terminal, a first terminal, and a second terminal.
- the control terminal is the gate electrode 1221
- the first terminal is the first electrode 1223
- the second terminal is the second electrode 1224.
- the switching element 122 further includes an active layer 1222.
- the gate electrode 1221 is disposed on the base substrate 11 and may use metal, transparent conductive material, or other suitable materials.
- the gate insulating layer 14 is provided on the base substrate 11 and covers the gate electrode 1221.
- the gate insulating layer 14 may use silicon nitride, silicon oxide, or other suitable materials.
- the active layer 1222 is provided on the gate insulating layer 14 for providing a channel region.
- Polysilicon semiconductor materials such as low-temperature polysilicon semiconductor materials, high-temperature polysilicon semiconductor materials, or other suitable materials, such as oxide semiconductor materials, can be used.
- indium zinc gallium oxide Indium Gallium Zinc Oxide, IGZO
- the embodiments of the present disclosure do not limit this.
- the first electrode 1223 and the second electrode 1224 are disposed on the gate insulating layer 14 and overlap the two ends of the active layer 1222.
- the first pole 1223 and the second pole 1224 may be symmetrically arranged, so the positions of the two can be interchanged.
- the first electrode 1223 is a source or a drain
- the second electrode 1224 is a drain or a source.
- the first pole 1223 and the second pole 1224 may use any suitable metals or alloys thereof, such as gold, silver, copper, aluminum, etc. The embodiments of the present disclosure do not limit this.
- the switching element 122 is not limited to the thin film transistor, but may also be a field effect transistor or other devices having similar characteristics.
- the switching element 122 may be a bottom gate thin film transistor or a top gate thin film transistor.
- the biochip 200 may further include film layers such as a light-shielding layer and a buffer layer. For the arrangement of these film layers, reference may be made to conventional designs, which will not be described in detail here.
- the working element 121 is provided on the passivation layer 15, and the passivation layer 15 covers the first pole 1223 and the second pole 1224 of the switching element 122.
- the working element 121 includes a metal electrode 1211 and an electric field controllable surface modification layer 1212 formed on the surface of the metal electrode 1211.
- the metal electrode 1211 is electrically connected to the second end (second electrode 1224) of the switching element 122 through the via 151 penetrating the passivation layer 15.
- the metal electrode 1211 may use gold, silver, or other suitable metals.
- the electric field controllable surface modification layer 1212 includes an electric field controllable isomerized organic molecule, and an end of the electric field controllable isomerized organic molecule is connected to the surface of the metal electrode 1211.
- the electric field controllable isomerization organic molecule may be a thioalcoholic acid (such as thiohexadecanoic acid, whose molecular structure is shown in FIG. 4) or a thioalcoholic acid derivative molecule.
- the thioalcoholic acid or thioalcoholic acid derivative molecule chemically bonds with the metal atom (or ion) in the metal electrode 1211 through the mercapto group at the end to form a covalent bond, thereby The thioalcoholic acid or thioalcoholic acid derivative molecules are attached to the surface of the metal electrode 1211.
- the flow channel 131 is disposed on the passivation layer 15 and includes oppositely disposed side walls 132.
- the U-shaped groove formed by the oppositely disposed side walls 132 and the passivation layer 15 constitutes the flow channel 131 and its multiple branches, thereby providing a flow channel for the fluid (eg, droplet) including the target substance.
- the working element 121 is located between the oppositely disposed side walls 132 so as to be in contact with the droplet including the target substance.
- the material of the side wall 132 may be a photosensitive organic material such as photoresist, which not only facilitates fabrication, but also has a low cost.
- the height of the flow channel 131 is 10 ⁇ m, and the width is 30 ⁇ m, that is, the height of the side wall 132 is 10 ⁇ m, and the distance between the opposite side walls 132 is 30 ⁇ m.
- the material of the side wall 132 is not limited to photosensitive organic materials such as photoresist, and other suitable materials may also be used.
- the height of the side wall 132 and the distance between the opposite side walls 132 The distance is not limited, the height of the side wall 132 is, for example, 8-12 ⁇ m, and the distance between the oppositely disposed side walls 132 is, for example, 25-35 ⁇ m, which can be determined according to actual needs.
- the side wall 132 is made by exposure development with photoresist (model: KMH-T546). For example, spin-coat a photoresist at a speed of 300 rpm on the passivation layer 15 (thermal weight loss temperature is 320 ° C), bake for 2 minutes before 90 ° C, repeat the spin coating once, and then expose through the mask to the target pattern and expose The intensity is 999mJ, the exposure time is 15 seconds, followed by development with a developer for 45 seconds, and curing at 230 ° C for 30 minutes, thereby obtaining the side wall 132.
- the height of the obtained side wall 132 is 9.8 ⁇ m. It should be noted that the above-mentioned process flow for manufacturing the side wall 132 is only exemplary, not limiting, and the side wall 132 may be manufactured by any suitable process.
- the gate 1221 of the switching element 122 is connected to a separately provided scan line (not shown in the figure), and the first pole 1223 of the switching element 122 is connected to a separately provided drive line (not shown in the figure) connection.
- the scanning line is used to apply a control signal to the gate 1221 (control terminal) of the switching element 122 to control the turning on or off of the switching element 122
- the driving line is used to apply an operating voltage to the first pole 1223 (first end) of the switching element 122 ), So that the switching element 122 applies the operating voltage to the operating element 121 according to the control signal.
- the switching element 122 when the control signal is valid, the switching element 122 turns on, transmits the operating voltage received by the first pole 1223 to the second pole 1224, and further transmits to the metal electrode 1211 of the operating element 121, and, by adjusting the drive line
- the magnitude of the transmitted working voltage can control the magnitude of the working voltage applied to the metal electrode 1211.
- the control signal is invalid, the switching element 122 is turned off, so the metal electrode 1211 of the working element 121 does not receive the working voltage. In this way, it is possible to determine whether to apply an operating voltage to the working element 121 according to the control signal, and the magnitude of the operating voltage can be adjusted.
- the scan line can also be connected to a separately provided control unit
- the drive line can also be connected to a separately provided control unit or a digitally controllable voltage source to receive the control signal and the operating voltage, respectively.
- the gates of the switching elements 122 in the same row can be made 1221 is connected to the same scanning line, so that the first poles 1223 of the same column of switching elements 122 are connected to the same driving line, thereby reducing the number of signal lines.
- the embodiments of the present disclosure are not limited to this, and the scanning line and the driving line may be separately provided for each switching element 122. In this way, each switching element 122 may be independently controlled and will not be affected by the same row or column The influence of the adjacent switching elements 122 in the circuit diversifies the combination of the on or off states of the plurality of switching elements 122.
- the biochip 200 may further include more or fewer components, and the relative positional relationship of each component is not limited, and may be determined according to actual needs.
- the biochip 200 may further include an opposite substrate, a buffer layer, a light-shielding layer, etc., to provide more abundant functions and improve the performance of the biochip 200.
- the working element 121 is in contact with the target substance 21, for example, and the target substance 21 can be fixed thereto.
- the target substance 21 is a gene fragment
- the gene fragment includes a functional fragment 211 and an end group 212.
- the functional fragment 211 may be an oligonucleotide, a primer, a probe, a target DNA fragment or a polypeptide, etc., which is not limited in the embodiments of the present disclosure.
- the functional fragment 211 when the functional fragment 211 is a probe, the functional fragment 211 may perform base complementary hybridization with the gene to be detected, thereby detecting the gene to be detected.
- the terminal group 212 is a sulfhydryl group, for example, it can be obtained by modifying the functional fragment 211 with cysteine (C 3 H 7 NO 2 S).
- the sulfhydryl group can chemically bond with the metal atom (or ion) of the metal electrode 1211 to form a covalent bond, thereby connecting the target substance 21 (ie, gene fragment) to the surface of the metal electrode 1211, To achieve the fixation of gene fragments.
- the end group of the gene fragment may further include one or more of amino group, hydroxyl group, carboxyl group, phosphate group, alkoxy group, amine group, fluorine-containing group, quaternary amino group and quaternary phosphorous group.
- the shape of the target substance 21 (that is, the gene fragment) shown in FIG. 5 is only schematic and does not represent the true shape of the gene fragment, and the size ratio of the end group 212 and the functional fragment 211 in the figure The relationship is only for a clearer description and explanation, but does not indicate the true size-to-size relationship.
- the electric field controllable surface modification layer 1212 can be obtained by modifying the metal electrode 1211 with electric field controllable isomerization organic molecules, that is, the electric field controllable surface modification layer 1212 includes electric field controllable isomerization organic molecules.
- the metal electrode 1211 is modified with thiohexadecanoic acid so that the mercapto group at the end of the thiohexadecanoic acid forms a covalent bond with the metal atom (or ion) in the metal electrode 1211, thereby The thiohexadecanoic acid is connected to the surface of the metal electrode 1211 to form an electric field controllable surface modification layer 1212.
- organic molecules with controlled electric field isomerization can include thioalcoholic acid (eg, thiohexadecanoic acid) or thioalcoholic acid derivative molecules, which have thiol groups at the ends to facilitate connection with the metal electrode 1211 .
- thioalcoholic acid eg, thiohexadecanoic acid
- thioalcoholic acid derivative molecules which have thiol groups at the ends to facilitate connection with the metal electrode 1211 .
- the types of organic molecules with controlled electric field isomerization are not limited, and may be molecules of any applicable substance.
- the groups at the ends of the organic molecules with controlled electric field isomerization are not limited to thiol groups, but can also be amino groups, hydroxyl groups, carboxyl groups, phosphate groups, alkoxy groups, amine groups, fluorine-containing groups, quaternary amine groups, quaternary phosphorus groups One or more of them are not limited in the embodiments of the present disclosure, and these groups can be connected to the metal electrode 1211 of a corresponding metal material to achieve corresponding functions.
- the hydrophilicity / hydrophobicity of the electric field controllable surface modification layer 1212 may vary according to the direction of the applied control electric field. For example, in one example, when the direction of the control electric field E applied to the electric field controllable surface modification layer 1212 is as shown by the arrow in FIG. 6A, the electric field controllable isomerization organic in the electric field controllable surface modification layer 1212 Molecules, for example, lie on the surface of the metal electrode 1211, thereby facilitating the flow of liquid. At this time, under the action of the control electric field E, the electric field controllable surface modification layer 1212 exhibits hydrophobicity.
- the target substance 21 will not contact the metal electrode 1211. And can flow on the electric field controllable surface modification layer 1212.
- the electric field controllable isomerization organic molecules in the electric field controllable surface modification layer 1212 stand on the surface of the metal electrode 1211, for example, This helps to retain liquid.
- the electric field controllable surface modification layer 1212 exhibits hydrophilicity. If the target substance 21 is located on the electric field controllable surface modification layer 1212, the target substance 21 may be in contact with the metal electrode 1211. And it is connected to the surface of the metal electrode 1211 through the mercapto group at the end.
- the positive and negative of the working voltage applied to the metal electrode 1211 can be controlled to form a control electric field E with a separately provided common electrode for providing a common voltage.
- the direction of the control electric field E is determined by the positive and negative of the working voltage and the common electrode
- the relative positional relationship with the metal electrode 1211 is determined.
- the action range of the control electric field E is not limited to the area where the metal electrode 1211 and the common electrode are directly opposed to each other, and the action range of the control electric field E can be expanded to the area where the metal electrode 1211 and the common electrode are directly opposed by controlling the magnitude of the operating voltage Outside the area. Therefore, the common electrode may be provided on the base substrate 11 below the working element 121, or may be provided on other components (such as the opposite substrate) opposite to the metal electrode 1211 than the base substrate 11.
- the first working unit 12_a and the second working unit 12_b are two adjacent working units located in the flow channel 131, and the droplet 20 is located in the flow channel 131 and includes the target substance 21.
- the droplet 20 can be driven from one working unit 12 to another working unit 12 (eg, from the first working unit 12_a to the second working unit 12_b) in a conventional electro-wetting manner, so that the droplet 20 can It flows between multiple work units 12 and can reach any one work unit 12.
- the operating voltage applied to the working element 121 of the working unit 12 adjacent to the droplet 20 to control the corresponding electric field controllable surface modification layer 1212 to exhibit hydrophilicity or hydrophobicity and control the hydrophilicity or hydrophobicity And control the polarity of the charge on the surface of the metal electrode 1211 of the adjacent working unit 12, so that the droplet 20 flows or is retained.
- a first voltage and an effective control signal are applied to the first switching element 122_a of the first working unit 12_a, so that the voltage of the first working element 121_a is the first voltage;
- the second switching element 122_b of the second working unit 12_b applies a second voltage and an effective control signal, so that the voltage of the second working element 121_b is the second voltage.
- the first voltage is a positive voltage
- the second voltage is a negative voltage and the absolute value of the negative voltage is small.
- the biochip 200 further includes a common electrode (not shown in the figure), the common electrode is disposed on the base substrate 11 and is located below the first working element 121_a and the second working element 121_b, and the common electrode is used to provide a common voltage
- a common electrode for example, non-metallic conductive materials such as indium zinc oxide, polysilicon, or suitable metal materials can be used.
- the direction of the control electric field E formed by the first working element 121_a is the same as the direction of the electric field shown in FIG. 6A
- the direction of the control electric field E formed by the second working element 121_b is the same as the direction of the electric field shown in FIG. 6B.
- the electric field controllable surface modification layer in the first working element 121_a exhibits hydrophobicity
- the electric field controllable surface modification layer in the second working element 121_b exhibits weak hydrophilicity.
- the surface of the metal electrode in the first working element 121_a accumulates positive charges under the action of the first voltage
- the side of the droplet 20 in contact with the first working element 121_a accumulates negative charge, and accordingly, the droplet 20 moves away from the first Positive charges accumulate on one side of the working element 121_a.
- the second working element 121_b accumulates negative charges under the action of the second voltage. Therefore, the side of the droplet 20 away from the first working element 121_a and the second working element 121_b have an attractive effect to promote the droplet 20 to roll. Thereby, the droplet 20 flows from the first working unit 12_a to the second working unit 12_b, so that the flow of the droplet 20 is realized. Since the hydrophilicity of the electric field controllable surface modification layer in the second working element 121_b is extremely weak, it will not affect the target substance 21 in the droplet 20.
- the plurality of electric field controllable surface modification layers 1212 located in the flow path of the droplet 20 as a whole show hydrophobicity, and pass the working voltage
- the droplet 20 can flow along the flow path.
- a negative voltage with a larger absolute value is applied to the working element 121, so that the corresponding electric field controllable surface modification layer 1212 exhibits hydrophilicity, thereby making the object in the droplet 20
- the substance 21 is fixed on the surface of the corresponding metal electrode 1211.
- the target substance 21 can be fixed on the predetermined working element 121, and the correspondence between the target substance 21 and the fixed position is clear.
- each working element 121 can be clearly known The sequence of the probes on the probe to facilitate subsequent detection and analysis.
- the positive and negative relationship and the magnitude relationship of the operating voltage applied to the working element 121 may be determined according to actual needs, and the embodiment of the present disclosure does not limit this, for example, according to the need to form the control
- the direction of the electric field E is determined as long as the flow of the droplet 20 can be controlled, and the target substance 21 in the droplet 20 can be fixed on the predetermined working element 121.
- the formation of droplets 20 can be achieved by adding a surfactant (eg, polyethylene glycol (PEG)) to the aqueous phase.
- a surfactant eg, polyethylene glycol (PEG)
- PEG polyethylene glycol
- the flow channel 131 of the biochip 200 may be filled with a 0.2% bovine serum albumin (BSA) solution and soaked for 1 hour to reduce the flow channel 131 After adsorbing the target substance 21 on the surface, the BSA solution can be pumped out by a micropump.
- BSA bovine serum albumin
- the active voltage applied to the working elements 121 of the plurality of working units 12 may be controlled by an active matrix composed of a plurality of switching elements 122, so that the droplet 20 containing the target substance 21 flows to the predetermined working element 121 by electrowetting on.
- a plurality of droplets 20 containing different target substances 21 are respectively flowed in different branches, and the flow paths of each other do not cross, so that a plurality of droplets 20 containing different target substances 21 can be simultaneously controlled It flows onto each predetermined working element 121. Using this multi-channel approach can effectively save time and cost.
- the biochip 200 can control the fixed position of the target substance 21 (that is, the gene fragment).
- the user only needs to know the position of the detection point to know the corresponding target substance 21 Sequence, convenient and fast.
- the fixed positions of different target substances 21 can also be separated from each other, so that after the target substances 21 are hybridized with the gene to be detected, the fluorescent crosstalk between the target substances 21 can be improved, and the detection accuracy can be improved. degree.
- the gene chip 200 facilitates subsequent image analysis and recognition, and helps increase detection throughput.
- the fixed position of the target substance 21 is controllable, the number of operation steps can be reduced.
- the sequencing step after the fixed gene fragment can be omitted compared to a chip that uses a microwell-bonded microsphere structure.
- the biochip 200 can also be fixed with primers for amplification and sequencing, and has a multifunctional function.
- the biochip 200 is compatible with a semiconductor manufacturing process. For example, it can be processed by a general manufacturing process of a display panel. The production cost is low, and it is suitable for mass production.
- different target substances 21 may be fixed on the plurality of working elements 121 to increase the detection flux.
- the first target substance 21_a, the second target substance 21_b, and the third target substance 21_c are fixed to the first working element 121_a, the second working element 121_b, and the third working element 121_c, respectively, and the first object
- the substance 21_a, the second target substance 21_b, and the third target substance 21_c are different from each other.
- the number of kinds of the target substance 21 may be less than or equal to the number of working elements 121. In the same biochip 200, the more kinds of the target substance 21, the larger the detection flux.
- FIG. 9 is a schematic cross-sectional view of another biochip provided by an embodiment of the present disclosure.
- the biochip 300 shown in FIG. 9 is similar to that shown in FIG. 3
- the biochip 200 is basically the same.
- the counter substrate 30 is opposite to the base substrate 11, and the working unit 12 is located between the counter substrate 30 and the base substrate 11.
- the opposite substrate 31 functions as support and protection, and it is convenient to provide the opposite electrode 32 on the opposite substrate 31.
- the counter base 31 may be a glass substrate, a plastic substrate, a quartz substrate, or a substrate made of other suitable materials, which is not limited in the embodiments of the present disclosure.
- the counter electrode 32 is provided on the surface of the counter base 31 opposed to the base substrate 11 and opposed to the working unit 12.
- the opposite electrode 32 is, for example, a common electrode for providing a common voltage to realize the formation of a control electric field between the opposite electrode 32 and the metal electrode 1211.
- the plurality of counter electrodes 32 corresponding to the plurality of working units 12 are connected as a whole, that is, the counter electrode 32 covers the area on the counter substrate 31 corresponding to the plurality of working units 12 to simplify the production process and facilitate processing .
- the counter electrode 32 may use any suitable material such as metal, transparent conductive material, etc. The embodiments of the present disclosure do not limit this.
- the side wall 132 abuts on the opposite substrate 30 to maintain the distance between the passivation layer 15 and the opposite substrate 30, and the side wall 132 may function to support the opposite substrate 30.
- the dielectric layer 33 is provided on the surface of the opposing electrode 32 opposite to the base substrate 11 and plays an insulating role.
- the dielectric layer 33 may be formed of silicon dioxide or the like.
- the hydrophobic layer 34 is disposed on the surface of the dielectric layer 33 opposite to the base substrate 11, and the hydrophobic layer 34 forms a closed space with the opposing sidewall 132 and the passivation layer 15 to form the flow channel 131 and its multiple branches To provide a flow path for the droplet 20. Since the flow channel 131 is closed, the biochip 300 is not easily affected by the environment and has strong anti-interference ability.
- the hydrophobic layer 34 has hydrophobicity to prevent the target substance 21 in the droplet 20 from adhering to its surface, causing waste of the target substance 21 and facilitating the flow of the droplet 20.
- the hydrophobic layer 34 may use any suitable material such as silicon nitride.
- the distance between the hydrophobic layer 34 and the passivation layer 15 is 10 ⁇ m.
- the working principle of the biochip 300 is similar to the working principle of the biochip 200.
- the first working unit 12_a and the second working unit 12_b are two adjacent working units located in the flow channel 131, and the droplet 20 is located in the flow channel 131 and includes the target substance 21.
- a third voltage and an effective control signal are applied to the first switching element 122_a of the first working unit 12_a, so that the voltage of the first working element 121_a is the third voltage; the second switching element 122_b of the second working unit 12_b
- the fourth voltage and the effective control signal are applied so that the voltage of the second working element 121_b is the fourth voltage.
- the third voltage is a negative voltage
- the fourth voltage is a positive voltage and the absolute value of the voltage is small.
- the common voltage is supplied to the opposite electrode 32, for example, ground.
- the direction of the control electric field E formed by the first working element 121_a is the same as the direction of the electric field shown in FIG. 6A
- the direction of the control electric field E formed by the second working element 121_b is the same as the direction of the electric field shown in FIG. 6B. Therefore, the electric field controllable surface modification layer in the first working element 121_a exhibits hydrophobicity, and the electric field controllable surface modification layer in the second working element 121_b exhibits weak hydrophilicity.
- the surface of the metal electrode in the first working element 121_a accumulates negative charge under the action of the third voltage
- the side of the droplet 20 that contacts the first working element 121_a accumulates positive charge, and accordingly, the droplet 20 moves away from the first Negative charge is accumulated on one side of the working element 121_a.
- the second working element 121_b accumulates positive charges under the action of the fourth voltage, so the side of the droplet 20 away from the first working element 121_a and the second working element 121_b have an attracting effect to promote the droplet 20 to roll. Thereby, the droplet 20 flows from the first working unit 12_a to the second working unit 12_b, so that the flow of the droplet 20 is realized. Since the hydrophilicity of the electric field controllable surface modification layer in the second working element 121_b is extremely weak, it will not affect the target substance 21 in the droplet 20.
- the target substance 21 in the droplet 20 is fixed on the surface of the metal electrode 1211 of the predetermined working element 121.
- the positive and negative relationship and the magnitude relationship of the operating voltage applied to the working element 121 may be determined according to actual needs, and the embodiment of the present disclosure does not limit this, for example, according to the need
- the direction of the electric field E is determined as long as the flow of the droplet 20 can be controlled.
- the biochip 300 can realize the controllability of the fixed position of the gene fragments, can improve the fluorescent crosstalk between the gene fragments and other problems, and is compatible with the semiconductor manufacturing process, the production cost is low, which helps to improve the detection accuracy and detection flux.
- At least one embodiment of the present disclosure also provides a biological detection system, including the biochip in any of the above embodiments of the present disclosure.
- the biological detection system can realize the controllability of the fixed position of the gene fragments, can improve the fluorescent crosstalk between the gene fragments and other problems, and is compatible with the semiconductor manufacturing process, the production cost is low, which helps to improve the detection accuracy and detection flux.
- the biodetection system 400 includes a biochip 401, which is a biochip in any embodiment of the present disclosure, such as the above-mentioned biochip 100/200/300.
- the biological detection system 400 further includes a control unit 410 configured to apply control signals to the plurality of working units 12 in the biochip 401.
- the control unit 410 may apply a control signal to cause the droplet 20 containing the target substance 21 to flow in the flow channel 131 of the biochip 401 and reach the predetermined working unit 12 and be fixed on the corresponding working element 121 to For the user to use the biochip 401 to detect the gene to be detected.
- control unit 410 can also be configured to provide an operating voltage without the need for an additional voltage source.
- control unit 410 may be implemented as dedicated or general-purpose electronic hardware (or circuit), which is not limited by the embodiments of the present disclosure.
- the specific configuration of the above electronic hardware is not limited, and may include analog devices, digital chips, or other suitable devices.
- At least one embodiment of the present disclosure also provides a method for manufacturing a biochip, by which the biochip in any of the above embodiments of the present disclosure can be manufactured.
- the manufacturing method By using the manufacturing method, the fixed position of the gene fragments can be controlled, the fluorescent crosstalk between the gene fragments can be improved, and the semiconductor preparation process is compatible, the production cost is low, and the detection accuracy and detection flux are improved.
- FIG. 12 is a schematic flowchart of a method for manufacturing a biochip according to an embodiment of the present disclosure.
- the manufacturing method of the biochip includes the following operations:
- Step S510 forming a plurality of working units 12 on the base substrate 11;
- Step S520 A control signal is applied to the selected working unit 12 of the plurality of working units 12, and a control electric field is formed by the working element 121 of the selected working unit 12, which controls the electric field of the working element 121 of the selected working unit 12
- the properties of the surface modification layer 1212 are controlled to control the operation of the fluid including the target substance 21.
- each working unit 12 includes a working element 121 for contacting with the target substance 21.
- the working element 121 includes a metal electrode 1211 and an electric field controllable surface modification layer 1212 formed on the surface of the metal electrode 1211.
- the operation of controlling the fluid including the target substance 21 includes: the fluid is driven through the selected working unit 12 or the target substance 21 in the fluid is fixed on the working element 121 of the selected working unit 12.
- At least one embodiment of the present disclosure also provides a method for operating a biochip.
- the biochip in any of the above embodiments of the present disclosure can be used.
- the fixed position of the gene fragments can be controlled, the fluorescent crosstalk between the gene fragments can be improved, and the semiconductor manufacturing process is compatible, the production cost is low, and the detection accuracy and detection flux are improved.
- the operation method of the biochip includes: applying a control signal to a selected working unit 12 of the plurality of working units 12, and forming a control electric field through the working element 121 of the selected working unit 12, which controls the selected working unit 12
- the electric field of the working element 121 can control the properties of the surface modification layer 1212 to control the operation of the fluid including the target substance 21.
- the operation of controlling the fluid including the target substance 21 includes: the fluid is driven through the selected working unit 12 or the target substance 21 in the fluid is fixed on the working element 121 of the selected working unit 12.
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Abstract
Description
Claims (18)
- 一种生物芯片,包括:衬底基板;多个工作单元,设置在所述衬底基板上;其中,每个所述工作单元包括配置为与对象物质接触的工作元件,所述工作元件包括金属电极和在所述金属电极的远离所述衬底基板且面向所述对象物质的表面的电场可控表面修饰层。
- 根据权利要求1所述的生物芯片,其中,所述电场可控表面修饰层包括电场可控异构化有机分子,所述电场可控异构化有机分子的端部连接到所述金属电极表面。
- 根据权利要求2所述的生物芯片,其中,所述电场可控异构化有机分子包括硫代醇酸或硫代醇酸衍生物分子,所述硫代醇酸或所述硫代醇酸衍生物分子通过端部的巯基连接到所述金属电极表面。
- 根据权利要求1-3任一所述的生物芯片,其中,所述金属电极的材料包括金和银中的至少之一。
- 根据权利要求1-4任一所述的生物芯片,还包括设置在所述衬底基板上的流道界定层,其中,所述流道界定层包括流道,所述对象物质的流体经所述流道到达所述多个工作单元中的至少之一。
- 根据权利要求5所述的生物芯片,其中,所述流道包括相对设置的侧壁,所述相对设置的侧壁构成多个支路,所述多个支路呈十字交叉且在交叉点处连通。
- 根据权利要求1-6任一所述的生物芯片,其中,每个所述工作单元还包括开关元件,所述开关元件包括控制端、第一端和第二端,所述工作元件与所述开关元件的第二端电连接,所述开关元件配置为根据控制信号确定是否对所述工作元件施加工作电压。
- 根据权利要求1-7任一所述的生物芯片,其中,所述衬底基板为玻璃基板。
- 根据权利要求1-8任一所述的生物芯片,其中,所述对象物质包括基因片段,所述基因片段固定在所述工作元件上。
- 根据权利要求9所述的生物芯片,其中,所述基因片段的端基包括巯基、氨基、羟基、羧基、磷酸酯基、烷氧基、胺基、含氟基团、季胺基和季磷基中的一种或多种。
- 根据权利要求1-10任一所述的生物芯片,还包括对置基板,其中,所述对置基板与所述衬底基板相对设置,所述工作单元位于所述对置基板和所述衬底基板之间。
- 根据权利要求11所述的生物芯片,其中,所述对置基板包括对置基底和对置电极,所述对置电极设置在所述对置基底的与所述衬底基板相对的表面上且与所述工作单元相对。
- 根据权利要求11或12所述的生物芯片,还包括设置在所述衬底基板上的流道界定层,其中,所述流道界定层包括流道,所述流道包括相对设置的侧壁,所述侧壁抵靠在所述对置基板上。
- 一种生物检测系统,包括控制单元,和如权利要求1-13任一所述的生物芯片,其中,所述控制单元配置为对所述生物芯片的所述多个工作单元施加控制信号。
- 一种生物芯片的制造方法,包括:在衬底基板上形成多个工作单元,其中,每个所述工作单元包括用于与对象物质接触的工作元件,所述工作元件包括金属电极和形成在所述金属电极的远离所述衬底基板且面向所述对象物质的表面的电场可控表面修饰层;对所述多个工作单元中的选定工作单元施加控制信号,通过所述选定工作单元的工作元件形成控制电场,所述控制电场控制所述选定工作单元的所述工作元件的电场可控表面修饰层的性质,以控制包括所述对象物质的流体的操作。
- 一种如权利要求1-13任一所述生物芯片的操作方法,包括:对所述多个工作单元中的选定工作单元施加控制信号,通过所述选定工作单元的工作元件形成控制电场,所述控制电场控制所述选定工作单元的所述工作元件的所述电场可控表面修饰层的性质,以控制包括所述对象物质的流体的操作。
- 根据权利要求16所述的操作方法,其中,所述控制电场使得所述电场可控表面修饰层中的电场可控异构化有机分子倒伏在所述金属电极的表面上,所述电场可控表面修饰层表现出疏水性,当所述对象物质位于所述 电场可控表面修饰层上时,所述对象物质与金属电极间隔,且所述对象物质在所述电场可控表面修饰层上流动。
- 根据权利要求16所述的操作方法,其中,所述控制电场使得所述电场可控表面修饰层中的电场可控异构化有机分子竖立在所述金属电极的表面上,所述电场可控表面修饰层表现出亲水性,当所述对象物质位于所述电场可控表面修饰层上时,所述对象物质与所述金属电极接触,且所述对象物质通过端部连接在所述金属电极的表面。
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CN112020551B (zh) | 2019-03-29 | 2022-11-25 | 京东方科技集团股份有限公司 | 检测芯片及其使用方法、反应系统 |
CN209974747U (zh) | 2019-04-09 | 2020-01-21 | 北京京东方技术开发有限公司 | 用于检测芯片的反应设备及反应系统 |
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CN109234158B (zh) | 2021-08-06 |
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