Digital microfluidic polymerase chain reaction multi-connection detection system

文档序号:641533 发布日期:2021-05-14 浏览:14次 中文

阅读说明:本技术 一种数字微流控聚合酶链式反应多联检测系统 (Digital microfluidic polymerase chain reaction multi-connection detection system ) 是由 苏阳 张研 于 2020-12-31 设计创作,主要内容包括:本发明提供一种数字微流控聚合酶链式反应多联检测芯片,通过控制体积调节电极实现液滴体积调节,可完成多个独立聚合酶链式反应,可搭配不同试剂实现不同的检测指标,扩增方法可采用基于可变温温度模块或温度恒定温度模块两种形式。在单个芯片上包含磁珠法核酸提取和聚合酶链式反应的功能,用户仅需要向芯片加载样品即可实现全流程全自动聚合酶链式反应多联检测,并可配合荧光检测模块实现定性或定量检测(即qPCR),还可通过电极设计或级联实现更高检测通量。(The invention provides a digital microfluidic polymerase chain reaction multi-connection detection chip, which can realize the volume adjustment of liquid drops by controlling a volume adjustment electrode, can finish a plurality of independent polymerase chain reactions, can be matched with different reagents to realize different detection indexes, and can adopt an amplification method based on a variable temperature module or a constant temperature module. The single chip comprises the functions of nucleic acid extraction by a paramagnetic particle method and polymerase chain reaction, a user can realize full-flow full-automatic polymerase chain reaction multi-joint detection only by loading a sample to the chip, qualitative or quantitative detection (namely qPCR) can be realized by matching with a fluorescence detection module, and higher detection flux can be realized by electrode design or cascade connection.)

1. A digital microfluidic polymerase chain reaction multi-joint detection chip comprises a plurality of sample/reagent inlets (1), a plurality of liquid storage areas (2), a waste liquid area (3), a stirring area (4), magnetic bead separation points (5), x mixing distribution areas (6), y row amplification areas (7) and volume adjusting electrodes (8);

wherein the chip realizes the volume adjustment of the liquid drop through the switch of the volume adjusting electrode (8);

a temperature module is also arranged below the chip amplification area and used for realizing temperature control so as to meet the temperature cycle condition required by the polymerase chain reaction;

the chip function comprises magnetic bead method nucleic acid extraction and polymerase chain reaction;

and x and y are positive integers greater than or equal to 1.

2. The digital microfluidic polymerase chain reaction multi-connected detection chip according to claim 1, wherein the chip is loaded on a detection device and filled with biocompatible medium oil;

preferably, a set of negative controls and/or a set of positive controls are included on the chip as internal controls;

preferably, the sample and/or the reagent can be loaded in a manner of injection by a pipette, loading by an independent reagent pack or pre-embedding the reagent in the chip;

preferably, the chip can be matched with different reagents to realize different detection indexes.

3. The digital microfluidic multiplex detection chip for polymerase chain reaction according to claim 1 or 2, wherein the temperature module is a variable temperature module (9), and the polymerase chain reaction is realized by changing the temperature of the variable temperature module (9), and each independent polymerase chain reaction solution does not need to move.

4. The digital microfluidic polymerase chain reaction multi-detection chip according to claim 1 or 2, wherein the temperature modules are constant temperature modules (10) and (11), and each independent polymerase chain reaction solution needs to move back and forth between two temperature intervals, so as to realize temperature cycling conditions required by polymerase chain reaction;

preferably, the temperature module (10) is kept constant, for example, at a constant denaturation temperature for carrying out denaturation reactions;

preferably, the temperature module (11) keeps, for example, a constant reverse transcription temperature for performing a reverse transcription reaction during a reverse transcription reaction stage, and is raised to, for example, a constant annealing and extension temperature for performing an annealing and extension reaction after the reverse transcription reaction is completed;

preferably, the denaturation temperature is 92-99 ℃, preferably 95 ℃;

preferably, the reverse transcription temperature is 45-75 ℃, preferably 50 ℃;

preferably, the annealing, extension temperature is 55-75 ℃, preferably 60 ℃.

5. A digital microfluidic multiplex detection system for polymerase chain reaction, which comprises the digital microfluidic polymerase chain reaction multiplex detection chip as claimed in any one of claims 1 to 4.

6. The digital microfluidic polymerase chain reaction multi-gang detection system of claim 5, wherein the system comprises a plurality of cascades of the chips to achieve higher detection throughput;

preferably, the system comprises a fluorescence detection module to enable qualitative or quantitative detection.

7. A method for multiplex PCR detection using the chip of any one of claims 1 to 4 or the system of claim 5 or 6, the method comprising:

(1) manually preparing a mixed solution of a sample, a lysis solution and magnetic beads, and oscillating to uniformly mix the mixed solution, wherein the manual reason is adopted in the step for ensuring the sufficient lysis of cells in the sample and the sufficient mixing of the cells and the magnetic beads;

(2) loading a chip on the detection equipment, filling the chip with biocompatible medium oil, and loading the mixed solution and various reagents of the first step at a corresponding inlet according to a specified volume;

(3) a mixing and distributing area (6) containing Master Mix 2X is fully mixed, n equal volumes of Master Mix 2X liquid drops are distributed and transferred to n positions close to the primer inlets;

(4) the mixing distribution area (6) containing deionized water is fully mixed, 2 drops of deionized water with the same volume are distributed under the condition that the volume adjusting electrode (8) is closed, and the drops are transferred to the positions close to the inlets of the negative control and the positive control of the primer;

(5) fully stirring a mixed solution of a sample, a lysis solution and magnetic beads in a stirring area (4), separating the magnetic beads at a magnetic bead separation point (5), fully stirring a washing solution and a rinsing solution with the magnetic beads in the stirring area (4) in sequence, separating the magnetic beads at the magnetic bead separation point (5), fully stirring an eluent and the magnetic beads in the stirring area (4), separating the magnetic beads at the magnetic bead separation point (5), and transferring the eluent to a mixing distribution area (6) containing deionized water;

(6) fully mixing a mixing distribution area (6) containing deionized water and eluent, distributing m drops with equal volume under the condition of opening a volume adjusting electrode (8), and transferring the drops to a position, close to a primer inlet, except for a negative control and a positive control of a primer, wherein the sum of the volumes of the drops of the deionized water and the negative or positive control in the step (4) is equal to the volume of the drops distributed in the step;

(7) fully mixing the n independent polymerase chain reaction solutions in the amplification area;

(8) and (3) amplifying the n independent polymerase chain reactions in the amplification area, and matching with a fluorescence detection device to realize fluorescence signal detection and result judgment.

8. The multiplex polymerase chain reaction detection method according to claim 7,

n and m are positive integers greater than or equal to 1;

preferably, the temperature control mode of the amplification zone adopts a temperature control mode based on the variable temperature module (9), n independent polymerase chain reaction solutions do not need to move, and the temperature cycling conditions required by the polymerase chain reaction are realized by changing the temperature of the variable temperature module (9).

9. The multiplex polymerase chain reaction detection method according to claim 7,

n and m are positive integers greater than or equal to 1;

preferably, the temperature control mode of the amplification zone can adopt a temperature control mode based on constant temperature modules (10) and (11), and n independent polymerase chain reaction solutions need to move back and forth between two temperature intervals, so as to realize the temperature cycling condition required by the polymerase chain reaction;

preferably, the temperature module (10) is kept constant, for example, at a constant denaturation temperature for carrying out denaturation reactions;

preferably, the temperature module (11) keeps, for example, a constant reverse transcription temperature for performing a reverse transcription reaction during a reverse transcription reaction stage, and is raised to, for example, a constant annealing and extension temperature for performing an annealing and extension reaction after the reverse transcription reaction is completed;

preferably, the denaturation temperature is 92-99 ℃, preferably 95 ℃;

preferably, the reverse transcription temperature is 45-75 ℃, preferably 50 ℃;

preferably, the annealing, extension temperature is 55-75 ℃, preferably 60 ℃.

10. The multiplex detection method for polymerase chain reaction according to any one of claims 7 to 9, wherein the method for digital microfluidic polymerase chain reaction multiplex detection further comprises a step of performing qualitative or quantitative detection (qPCR) by using a fluorescence detection module;

preferably, the method for digital microfluidic polymerase chain reaction multiplex detection further comprises using an electrode design or cascade to achieve higher detection throughput.

Technical Field

The invention belongs to the technical field of digital microfluidic control, and relates to a digital microfluidic polymerase chain reaction multi-connection detection system.

Background

Polymerase Chain Reaction (PCR) is the most commonly used experimental method for nucleic acid detection, and its basic process is: after the detection sample is combined with the reaction reagent, firstly, reverse transcription reaction and pre-denaturation reaction are carried out, and then, 30-50 times of temperature cycle is carried out between deformation reaction temperature and annealing and extension reaction temperature to realize the copy of the target nucleic acid fragment. The traditional detection means of PCR detects the amplification result of target nucleic acid fragments in a nucleic acid electrophoresis mode after all temperature cycles are finished, and the current detection means which is more commonly used is to add a fluorescent probe into a PCR detection reagent and detect the fluorescence signal intensity of a reaction solution after all temperature cycles or after each temperature cycle is finished by using a fluorescence detection device so as to detect the amplification result of the target nucleic acid fragments. At present, commercial PCR detection equipment is mainly used in cooperation with 96-well plates and 384-well plates, for example, a detection sample and a reagent are mixed and then added into a reaction well of the well plate, a high-precision temperature change module is used for realizing temperature circulation, and a fluorescence detection device is used for judging results. The multiplex detection of the polymerase chain reaction is an important detection means, has very important application value particularly in the aspects of detection of respiratory viruses and bacteria, the main means for realizing the multiplex detection of the polymerase chain reaction still depends on manual operation at present, and the Filmarray product of Biofire and the ePLex product of Genmark respectively utilize a microfluidic technology to realize full-flow full-automatic multiplex detection of the polymerase chain reaction, thereby greatly improving the detection efficiency.

The main defects of the traditional manual operation are that the detection efficiency is low, the detection is long in time consumption, a professional detection laboratory and a professional technician are required to complete the detection, and the detection result is unreliable due to the risks of experiment failure or sample pollution caused by misoperation of an operator in the detection process. The Filmar ray product of Biofire adopts a pressure type microfluidic chip to realize full-flow full-automatic polymerase chain reaction multi-link detection, but the cost is high due to the complex manufacturing process of the chip, and the price expectation of the detection method in the market is difficult to achieve. The detection means of the ePLex product of Genmark adopts electrochemical gene hybridization instead of polymerase chain reaction generally accepted by the industry, the reliability of the detection result is not as good as that of the polymerase chain reaction, and the defects of high chip manufacturing cost exist.

Therefore, there is a need to provide a new multi-connected detection system with high integration level, low cost and high reliability for full-automatic digital microfluidic polymerase chain reaction, and the system has a wide application prospect and a huge market value in the technical field of nucleic acid detection based on polymerase chain reaction.

Disclosure of Invention

Aiming at the defects and practical requirements of the prior art, the invention provides a digital microfluidic Polymerase Chain Reaction (PCR) multiplex detection system. The single chip comprises a nucleic acid extraction function of a sample by a magnetic bead method, a plurality of independent PCR or qPCR reactions and 1 group of negative and positive control reactions can be accommodated, and a user can realize full-flow full-automatic polymerase chain reaction multi-joint detection only by loading the sample to the chip.

In order to achieve the purpose, the invention adopts the following technical scheme:

in a first aspect, the invention provides a digital microfluidic polymerase chain reaction multi-link detection chip, which mainly comprises a plurality of sample/reagent inlets 1, a plurality of liquid storage areas 2, a waste liquid area 3, a stirring area 4, magnetic bead separation points 5, x mixed distribution areas 6, y rows of amplification areas 7 and volume adjusting electrodes 8; x and y are positive integers greater than or equal to 1;

preferably, the chip is loaded on the detection device and filled with biocompatible medium oil;

preferably, the chip realizes the adjustment of the volume of the liquid drop through the volume adjusting electrode 8;

preferably, a set of negative controls and/or a set of positive controls are included on the chip as internal controls;

preferably, the sample and reagent loading positions are as shown in FIG. 2;

preferably, the reagent can be loaded in a manner of injection by a pipette, loading by an independent reagent pack or pre-embedding in a chip;

preferably, the chip can be matched with different reagents to realize different detection indexes;

preferably, the chip functions comprise magnetic bead nucleic acid extraction and polymerase chain reaction;

preferably, a temperature module is further configured below the chip amplification region, and is used for realizing temperature control so as to meet temperature cycling conditions required by polymerase chain reaction;

in one embodiment, the temperature module is a temperature-changing temperature module 9, and the temperature-changing temperature module 9 can enable the temperature control manner of the amplification zone to adopt a temperature-changing temperature control manner as shown in fig. 5, in which n independent polymerase chain reaction solutions do not need to move, and amplification is achieved by changing the temperature of the temperature-changing temperature module 9 to achieve the temperature cycling conditions required by the polymerase chain reaction;

in another embodiment, the temperature modules are constant temperature modules 10 and 11, each of the separate pcr solutions needs to be moved back and forth between two temperature intervals to achieve the desired temperature cycling conditions for the pcr;

preferably, the temperature module 10 is kept constant, for example, at a constant denaturation temperature for carrying out denaturation reactions;

preferably, the temperature module 11 keeps, for example, a constant reverse transcription temperature for performing a reverse transcription reaction during a reverse transcription reaction stage, and is raised to, for example, a constant annealing and extension temperature for performing an annealing and extension reaction after the reverse transcription reaction is completed;

preferably, the denaturation temperature is 92-99 ℃, preferably 95 ℃;

preferably, the reverse transcription temperature is 45-75 ℃, preferably 50 ℃;

preferably, the annealing, extension temperature is 55-75 ℃, preferably 60 ℃.

In a second aspect, the invention provides a digital microfluidic multiplex polymerase chain reaction detection system, which comprises the digital microfluidic polymerase chain reaction multiplex detection chip of the first aspect.

Preferably, the digital microfluidic polymerase chain reaction multi-joint detection system comprises a fluorescence detection module, and can realize qualitative or quantitative detection (namely qPCR);

preferably, the digital microfluidic polymerase chain reaction multiplex detection system comprises an electrode design or cascade to achieve higher detection throughput.

In a third aspect, the present invention provides a method for multiplex detection of polymerase chain reaction using the chip of the first aspect or the system of the second aspect, the method comprising:

(1) manually preparing a mixed solution of a sample, a lysis solution and magnetic beads, and oscillating to uniformly mix the mixed solution, wherein the manual reason is adopted in the step for ensuring the sufficient lysis of cells in the sample and the sufficient mixing of the cells and the magnetic beads;

(2) loading a chip on the detection equipment, filling the chip with biocompatible medium oil, and loading the mixed solution and various reagents of the first step at corresponding inlets according to the volume in the figure 2;

(3) a mixing and distributing area 6 containing Master Mix 2X is used for fully mixing and distributing n equal-volume Master Mix 2X liquid drops and transferring the liquid drops to n positions close to the primer inlets;

(4) fully mixing the mixture distribution area 6 containing the deionized water, distributing 2 drops of deionized water with the same volume under the condition of closing the volume adjusting electrode 8, and transferring the drops to positions close to the inlets of the negative control and the positive control of the primer;

(5) fully stirring a mixed solution of a sample, a lysis solution and magnetic beads in a stirring area 4, separating the magnetic beads at a magnetic bead separation point 5, fully stirring a washing solution and a rinsing solution with the magnetic beads in the stirring area 4 in sequence, separating the magnetic beads at the magnetic bead separation point 5, fully stirring an eluent and the magnetic beads in the stirring area 4, separating the magnetic beads at the magnetic bead separation point 5, and transferring the eluent to a mixing and distributing area 6 containing deionized water;

(6) fully mixing the mixed distribution area 6 containing the deionized water and the eluent, distributing m drops of liquid drops with the same volume under the condition of starting the volume adjusting electrode 8, and transferring the drops to the positions, close to the primer inlets, of the negative control and the positive control except the primers, wherein the sum of the volumes of the drops of the deionized water and the negative or positive control in the step (4) is equal to the volume of the drops distributed in the step;

(7) fully mixing the n independent polymerase chain reaction solutions in the amplification area;

(8) and (3) amplifying the n independent polymerase chain reactions in the amplification area, and matching with a fluorescence detection device to realize fluorescence signal detection and result judgment.

Wherein n and m are positive integers greater than or equal to 1;

in one embodiment, the temperature control manner of the amplification region may be a temperature control manner based on the temperature-variable temperature module 9 as shown in fig. 5, in which n independent pcr solutions do not need to move, and the amplification is realized by changing the temperature of the temperature-variable temperature module 9 to realize the temperature cycling conditions required by the pcr;

in another embodiment, the temperature control manner of the amplification zone can be a temperature control manner based on two temperature-constant temperature modules 10 and 11 as shown in FIG. 6, and n independent PCR solutions need to be moved back and forth between two temperature intervals, so as to realize the temperature cycling conditions required by the PCR;

preferably, the temperature module 10 is kept constant, for example, at a constant denaturation temperature for carrying out denaturation reactions;

preferably, the temperature module 11 keeps, for example, a constant reverse transcription temperature for performing a reverse transcription reaction during a reverse transcription reaction stage, and is raised to, for example, a constant annealing and extension temperature for performing an annealing and extension reaction after the reverse transcription reaction is completed;

preferably, the denaturation temperature is 92-99 ℃, preferably 95 ℃;

preferably, the reverse transcription temperature is 45-75 ℃, preferably 50 ℃;

preferably, the annealing, extension temperature is 55-75 ℃, preferably 60 ℃.

Preferably, the method for the multiplex detection of the digital microfluidic polymerase chain reaction further comprises the step of realizing qualitative or quantitative detection (namely qPCR) by adopting a fluorescence detection module;

preferably, the method for digital microfluidic polymerase chain reaction multiplex detection further comprises using an electrode design or cascade to achieve higher detection throughput.

Compared with the prior art, the invention has the following beneficial effects:

(1) the full-flow full-automatic digital microfluidic chip provided by the invention replaces manual operation, so that the detection efficiency and accuracy are greatly improved, and the detection method is short in time consumption, low in cost and high in reliability;

(2) the chip type totally-enclosed detection environment has no pollution risk and high flexibility, and is suitable for detection of various indexes;

(3) the digital microfluidic polymerase chain reaction multi-link detection system has high expansibility, can realize higher detection flux through electrode design or cascade, has high integration level, and can realize customized experiment process.

Drawings

Fig. 1 is a schematic diagram of a digital microfluidic polymerase chain reaction multiplex detection chip, which mainly comprises a plurality of sample/reagent inlets 1, a plurality of liquid storage regions 2, a waste liquid region 3, a stirring region 4, magnetic bead separation points 5, x mixing distribution regions 6, y amplification regions 7 and volume adjustment electrodes 8; and x and y are positive integers greater than or equal to 1.

FIG. 2 is a schematic view of a sample and reagent loading position.

FIG. 3 is a schematic diagram of a digital microfluidic polymerase chain reaction multiplex detection operation.

Fig. 4 is a schematic diagram of the switching state of the volume adjustment electrode 8.

Fig. 5 is a schematic diagram of a digital microfluidic polymerase chain reaction multiplex detection system based on a variable temperature module 9.

Fig. 6 is a schematic diagram of a digital microfluidic polymerase chain reaction multi-connection detection system based on two temperature-constant temperature modules 10 and 11.

Detailed Description

To further illustrate the technical means adopted by the present invention and the effects thereof, the present invention is further described below with reference to the embodiments and the accompanying drawings. It is to be understood that the specific embodiments described herein are merely illustrative of the invention and are not limiting of the invention.

The examples do not show the specific techniques or conditions, according to the technical or conditions described in the literature in the field, or according to the product specifications. The reagents or apparatus used are conventional products commercially available from normal sources, not indicated by the manufacturer.

Example 1: polymerase Chain Reaction (PCR) multiplex detection of 13 detection indexes of 1 sample

Fig. 1 is a schematic diagram of a digital microfluidic polymerase chain reaction multiplex detection chip, which mainly comprises a plurality of sample/reagent inlets 1, a plurality of liquid storage regions 2, a waste liquid region 3, a stirring region 4, magnetic bead separation points 5, x mixing distribution regions 6, y amplification regions 7 and volume adjustment electrodes 8; and x and y are positive integers greater than or equal to 1. The polymerase chain reaction multiple detection of 13 detection indexes of 1 sample comprises the following steps:

(1) manually preparing a mixed solution of a sample, a lysis solution and magnetic beads, and oscillating to uniformly mix the mixed solution, wherein the manual reason is adopted in the step for ensuring the sufficient lysis of cells in the sample and the sufficient mixing of the cells and the magnetic beads;

(2) loading a chip on the detection equipment, filling the chip with biocompatible medium oil, and loading the mixed solution and various reagents of the first step at corresponding inlets according to the volume in the figure 2;

(3) a mixing and distributing area 6 containing Master Mix 2X is used for fully mixing and distributing n equal-volume Master Mix 2X liquid drops and transferring the liquid drops to n positions close to the primer inlets;

(4) the mixing distribution area 6 containing deionized water is fully mixed, 2 drops of deionized water with the same volume are distributed under the condition that the volume adjusting electrode 8 is closed, and the drops are transferred to the positions close to the inlets of the negative control and the positive control of the primer;

(5) fully stirring a mixed solution of a sample, a lysis solution and magnetic beads in a stirring area 4, separating the magnetic beads at a magnetic bead separation point 5, fully stirring a washing solution and a rinsing solution with the magnetic beads in the stirring area 4 in sequence, separating the magnetic beads at the magnetic bead separation point 5, fully stirring an eluent and the magnetic beads in the stirring area 4, separating the magnetic beads at the magnetic bead separation point 5, and transferring the eluent to a mixing and distributing area 6 containing deionized water;

(6) fully mixing the mixed distribution area 6 containing the deionized water and the eluent, distributing m drops of liquid drops with the same volume under the condition of starting the volume adjusting electrode 8, and transferring the drops to the positions, close to the primer inlets, of the negative control and the positive control except the primers, wherein the sum of the volumes of the drops of the deionized water and the negative or positive control in the step (4) is equal to the volume of the drops distributed in the step;

(7) fully mixing the n independent polymerase chain reaction solutions in the amplification area;

(8) and (3) amplifying the n independent polymerase chain reactions in the amplification area, and matching with a fluorescence detection device to realize fluorescence signal detection and result judgment.

Example 2: digital microfluidic polymerase chain reaction multi-connection detection based on variable temperature module 9

A temperature module is arranged below the chip amplification area and used for realizing temperature control so as to meet the temperature cycling condition required by the polymerase chain reaction.

The temperature control manner of the amplification zone can adopt a temperature control manner based on the temperature-variable temperature module 9 as shown in fig. 5, and under the temperature control manner, n independent polymerase chain reaction solutions do not need to move, and the temperature circulation conditions required by the polymerase chain reaction are realized by changing the temperature of the temperature-variable temperature module 9, so that the amplification is realized.

Example 3: digital microfluidic polymerase chain reaction multi-connection detection based on two temperature constant temperature modules 10 and 11

A temperature module is arranged below the chip amplification area and used for realizing temperature control so as to meet the temperature cycling condition required by the polymerase chain reaction.

The temperature control of the amplification section may be performed by a temperature control method based on two temperature-constant temperature modules 10 and 11 as shown in FIG. 6, in which the temperature module 10 is kept at, for example, 95 ℃ for performing the denaturation reaction, and the temperature module 11 is kept at, for example, 50 ℃ during the reverse transcription reaction, and is increased to, for example, 60 ℃ after the reverse transcription reaction is completed for performing the annealing and extension reactions. The n independent polymerase chain reaction solutions need to move back and forth between two temperature intervals, so that the temperature cycling conditions required by the polymerase chain reaction are realized, and the amplification is realized.

Example 4: high throughput assay

The digital microfluidic polymerase chain reaction multi-joint detection system realizes higher detection flux through electrode design or cascade connection, and can be matched with different reagents to realize different detection indexes.

In summary, the full-flow full-automatic digital microfluidic multiplex detection chip for polymerase chain reaction of the present invention can complete multiple independent polymerase chain reactions by controlling the volume adjustment electrode to achieve the volume adjustment of the droplets, and can be matched with different reagents to achieve different detection indexes, and the amplification method can adopt two forms based on a variable temperature module or a constant temperature module. The chip functions comprise magnetic bead nucleic acid extraction and polymerase chain reaction, qualitative or quantitative detection (namely qPCR) can be realized by matching with a fluorescence detection module, and higher detection flux can be realized by electrode design or cascade. The digital microfluidic chip provided by the invention replaces manual operation, so that the detection efficiency and accuracy are greatly improved, the detection method is short in time consumption, low in cost and high in reliability, and the chip type totally-enclosed detection environment is free from pollution risks.

The applicant states that the present invention is illustrated in detail by the above examples, but the present invention is not limited to the above detailed methods, i.e. it is not meant that the present invention must rely on the above detailed methods for its implementation. It should be understood by those skilled in the art that any modification of the present invention, equivalent substitutions of the raw materials of the product of the present invention, addition of auxiliary components, selection of specific modes, etc., are within the scope and disclosure of the present invention.

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