Specific primer and test kit for detecting pathogenic variation of deafness gene based on multiplex PCR and high-throughput sequencing technology and application

A technology of technical detection and deafness gene, which is applied in the field of genetic detection, can solve problems such as time-consuming and laborious, high technical requirements, and restrictions on wide application, and achieve the effects of reducing costs, simplifying operation steps, and improving detection efficiency

Active Publication Date: 2020-11-24
郑州桑林生物科技有限公司 +1
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0009] One-generation sequencing is the traditional method for genetic testing of hereditary deafness, and is the gold standard for genetic testing; however, this technology is time-consuming, laborious, low-throughput and high-priced, which limits its clinical application
The microarray chip diagnostic technology combined with deafness genes can quickly obtain results, but the method contains a limited number of genes and loci, and cannot detect rare variants carried by patients, resulting in many patients being undiagnosed
Denaturing high performance liquid chromatography has the characteristics of high automation and low detection cost, and can detect multiple mutation sites at the same time, but its technical requirements are high and special instruments are required, which limits its clinical application, and is now mostly used in laboratory detection
Time-of-flight mass spectrometry has a high throughput. Each instrument can detect 3000 samples per day. It can detect many sites and is efficient and accurate. However, it requires high personnel skills and the purity of the test samples, and the instrument is expensive, so it is not suitable for Generally carried out by medical institutions, which limits its wide application

Method used

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  • Specific primer and test kit for detecting pathogenic variation of deafness gene based on multiplex PCR and high-throughput sequencing technology and application
  • Specific primer and test kit for detecting pathogenic variation of deafness gene based on multiplex PCR and high-throughput sequencing technology and application
  • Specific primer and test kit for detecting pathogenic variation of deafness gene based on multiplex PCR and high-throughput sequencing technology and application

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0030] Example 1 uses specific primers to amplify the target region:

[0031] Since the primer amplification regions are too close or overlap each other, they need to be divided into two primer pools for PCR respectively. The primers are library amplification primer I (18 pairs of primers) and library amplification primer II (16 pairs of primers).

[0032] Thaw deafness-specific primers I, deafness-specific primers II, multiplex PCR enzyme mixture, positive quality control (PC), negative quality control (NC) and blank quality control (BC) and mix them upside down ten times after thawing , centrifuge briefly, and store on ice for later use.

[0033] 1) DNA template preparation: quantify the extracted nucleic acid to 1-10ng / μl, and the final volume is greater than 11μl;

[0034] 2) Take the deafness-specific primer I and multiple PCR enzyme mixture in a PCR tube to prepare the following reaction (denoted as: library amplification product 1):

[0035] Note: Take 5.5 μl each of th...

Embodiment 2

[0044] Example 2 Amplified product end repair, universal primer and Index connection

[0045] 1) In this step, the adapter will be connected to the end of the PCR product. After thawing the amplification enzyme mixture, the universal end adapter and the required index adapter, invert it up and down ten times to mix well, centrifuge briefly, and put it on ice for later use;

[0046] 2) Prepare the following reaction in a new PCR tube (marked as: PCR Mix tube):

[0047]

[0048] 3) Use a pipette to blow and mix 10 times, and place in a palm centrifuge for 5 seconds;

[0049] 4) Transfer the two tubes of reaction solutions of library amplification product 1 and library amplification product 2 to PCR Mix tubes in sequence, mix well by blowing and blowing for 10 times with a pipette, and centrifuge in a palm centrifuge for 5 seconds;

[0050] 5) Put the PCR tube in the PCR instrument and perform the following reaction:

[0051]

[0052]

[0053] 6) After the amplificatio...

Embodiment 3

[0054] Example 3 Purification

[0055] Purify the reaction product using the recommended purification beads Vazyme DNA Clean Beads:

[0056] 1) After the magnetic beads are equilibrated to room temperature, vortex to mix the DNA Clean Beads;

[0057] 2) According to the ratio of 1:0.8, pipette 64μl DNA Clean Beads into 80μl PCR product, vortex or use a pipette to gently pipette 10 times to mix thoroughly;

[0058] 3) Incubate at room temperature for 5 minutes;

[0059] 4) Centrifuge the PCR tube in a palm centrifuge for 5 seconds and place it in a magnetic stand to separate the magnetic beads and liquid. After the solution is clarified (about 5 minutes), carefully remove the supernatant;

[0060] 5) Keep the PCR tube always placed in the magnetic stand, add 180 μl of freshly prepared 80% ethanol to rinse the magnetic beads, incubate at room temperature for 30 seconds, and carefully remove the supernatant;

[0061] 6) Repeat the above step 5), rinse twice in total;

[0062]...

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Abstract

The invention relates to a specific primer and a test kit for detecting pathogenic variation of a deafness gene based on multiplex PCR and a high-throughput sequencing technology and application. Mosthereditary deafness can be subjected to high-efficiency, low-cost and comprehensive diagnosis; the specific primer and the test kit can also be used for newborn screening and early detection early treatment and can reduce matte caused by deafness, and the technical scheme for solving the problem is as follows: the multiplex PCR specific primer comprises 34 pairs of specific primers which are divided into two Pools, and Pool-1 comprises 18 pairs of primers, wherein the nucleic acid sequences are shown as SEQ ID NO: 1 to SEQ ID NO: 36; pool-2 comprises 16 pairs of primers, and the nucleotide sequence is shown as SEQ ID NO.37-68. According to the specific primer, the detection efficiency and accuracy can be effectively improved, the cost is reduced, the operation steps are simplified, and the specific primer is an innovation of specific primers for detecting the pathogenic variation of the deafness gene.

Description

technical field [0001] The invention relates to the field of gene detection, in particular to a specific primer, kit and application for detecting pathogenic variants of deafness genes based on multiplex PCR and high-throughput sequencing technology. Background technique [0002] Deafness is one of the most common disabilities, which can seriously affect human cognition and communication. There are as many as 360 million hearing-impaired people worldwide (WHO, 2017). About 1 in 500 newborns is affected by hearing loss. In China, there are about 800,000 hearing-impaired children under the age of 7, and this number is increasing at a rate of 30,000 cases every year. Non-syndromic or syndromic deafness associated with genetic factors accounts for about 60%. Non-synthetic deafness usually refers to deafness without other clinical symptoms, accounting for 70% of hereditary deafness. About 80% of sensorineural deafness is autosomal recessive (AR), besides, close to 20% of deafn...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/6883C12Q1/6869C12N15/11
CPCC12Q1/6883C12Q1/6869C12Q2600/156C12Q2531/113C12Q2537/143C12Q2535/122Y02A50/30
Inventor 汤文学许红恩杨增光刘欢飞李瑞君张娟丽于婷郭建成郭永军田永安
Owner 郑州桑林生物科技有限公司
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