Method for constructing high-throughput sequencing library of immune group library for screening cross-reaction between samples

A technology of cross-reaction and immune group library, which is applied to the determination/testing of microorganisms, biochemical equipment and methods, etc., which can solve the complex reaction system, multi-primer reaction that cannot achieve equivalent amplification, and cannot fully capture alleles And other issues

Pending Publication Date: 2019-09-20
NANFANG HOSPITAL OF SOUTHERN MEDICAL UNIV
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AI Technical Summary

Problems solved by technology

[0005] Although next-generation sequencing technology can quickly and high-throughput scan the immune repertoire in a panoramic manner, there are still obvious shortcomings in the two current methods.
1. The multiplex PCR method uses a variety of primers, and the reaction system is extremely complicated; the design of multiplex primers can only be designed based on known reference sequences, and cannot completely capture all alleles in the human immune repertoire; multiple primer reactions cannot To achieve equivalent amplification, the different amplification efficiencies between different primers lead to the existence of PCR bias, which makes the results quite different from the real situation
2. Although the simple 5`RACE method can achieve equivalent amplification, it cannot distinguish cross-reactions between samples when building a library
3. In the two amplification methods, chimera sequence products exist and occupy a considerable proportion, but the existing technology and analysis methods cannot identify most of the cross-product sequences, which will interfere with our sample sequences , resulting in a sequence error between samples

Method used

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  • Method for constructing high-throughput sequencing library of immune group library for screening cross-reaction between samples
  • Method for constructing high-throughput sequencing library of immune group library for screening cross-reaction between samples
  • Method for constructing high-throughput sequencing library of immune group library for screening cross-reaction between samples

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0077] Example 1 1ml Human Peripheral Blood Sample Immune Repertoire High-throughput Sequencing Library Construction Method

[0078] 1. Preparation of cDNA template

[0079] (1) 1ml of human peripheral blood was collected using EDTA anticoagulant tubes, and density gradient centrifugation was used to separate blood from

[0080] For mononuclear cells, add 600ul cell lysate for cell lysis, and use RNA extraction kit for RNA extraction.

[0081] (2) Detect the integrity of RNA and measure the concentration of RNA.

[0082] (3) Configure the mixed system according to the following table 5, and carry out the reaction on the PCR instrument. The reaction program is: 70°C, 1min,

[0083] Immediately after the completion of the reaction program, the product was placed on ice for 3 min. table 5

[0084]

[0085] (4) Configure the mixing system in Table 6 below, mix it with the product of step (3) and put it on the PCR instrument for reaction. The reaction program is: 42°C, 90min...

Embodiment 2

[0102] Example 2: Construction of high-throughput sequencing library of immune repertoire of 1mg human breast cancer tissue sample

[0103] 1. Preparation of cDNA template

[0104] (1) Take out human breast cancer tissue samples from liquid nitrogen or -80°C refrigerator, weigh 1 mg, grind the tissue into powder by liquid nitrogen grinding method, add 600ul cell lysate for cell lysis, use RNA extraction kit for RNA extraction.

[0105] (2) Detect the integrity of RNA and measure the concentration of RNA.

[0106](3) Configure the mixed system according to the following Table 10, and carry out the reaction on the PCR instrument. The reaction program is: 70°C, 1 min. After the reaction program is completed, immediately put the product on ice for 3 min.

[0107] Table 10

[0108]

[0109] (4) Configure the mixing system in Table 11 below, mix it with the product of step (3) and put it on the PCR instrument for reaction. The reaction program is: 42°C, 90min, 75°C, 15min, 4°C...

Embodiment 3

[0128] (1) Identify the problem sequence in the sample by adding the sequence of double-ended barcode. According to the known barcode sequence combination, remove the barcode combination sequence that does not exist theoretically in the sequencing data to improve the accuracy of each sample sequence source. The data of the 14 libraries used for testing are shown in Table 15 and figure 2 Shown:

[0129] Table 15:

[0130]

[0131]

[0132] surface figure 2 :

[0133]

[0134] Through Table 15 and Table figure 2 From the results in the table, it can be seen that 15% to 40% of the sequences in the sequencing samples do not follow the Barcode sequence combination number of the sample theory, and this part of the sequence will cause certain error interference to the analysis and quantification of the subsequent antibody library. Through the technical application of the present invention, we can remove this part of the wrong sequence and improve the accuracy of the a...

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Abstract

The invention relates to a method for constructing a high-throughput sequencing library of an immune group library for screening a cross-reaction between samples. The method is characterized in that: RNA of more than 10 ng is taken as a starting amount, a principle of RACE is used to make the template conversion when the RNA is reversely transcribed into cDNA, a known sequence is added to the 5' ends of all cDNAs, a product with the known sequence is used as a template, PCR amplification is performed by using a double-ended Barcode primer, the resulting product is purified and ligated to a sequencing linker sequence to obtain the final sequencing library, which can be used for samples of different receptor sources, during PCR amplification, PCR amplification can be performed using only one pair of primers to achieve equivalent amplification, and the primer preference problem caused by multiplex primer amplification is solved, and the upstream and downstream primers used in PCR amplification are designed to be labeled with Barcode composed of 4 to 12 different bases, which avoids the problem of cross-reaction between samples when multiple samples are simultaneously constructed.

Description

technical field [0001] The invention belongs to the field of biomedical services, and in particular relates to a PCR amplification of human immune repertoire, library construction and application in next-generation sequencing, especially a high-throughput sequencing of an immune repertoire for screening cross-reactions between samples Library construction method. Background technique [0002] The immune system is mediated by the surface receptors of immune B cells and T cells, and binds to pathogens or antigens derived from pathogens, and then exerts immune functions to protect the body from infringement. BCR immunoglobulin heavy chain (IGH) and TCR beta chain (TCRB) generate combinatorial diversity through rearrangement of V gene, D gene and J gene segments. At the junction between V-D and D-J, deletion of nucleotides and random addition of nucleotide sequences generated diversity in receptor junctions. The light chains produced by antibody immunization, immunoglobulin la...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/6806C12Q1/6869
CPCC12Q1/6806C12Q1/6869C12Q2525/191C12Q2535/122
Inventor 张镇海何奖图蓝春红王敏惠朱燕李丽敏
Owner NANFANG HOSPITAL OF SOUTHERN MEDICAL UNIV
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