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Library building method for screening large samples of thalassemia based on high-throughput sequencing

A thalassemia, high-throughput technology, applied in biochemical equipment and methods, chemical libraries, microbial measurement/testing, etc., can solve the problems of inapplicable large-scale screening, few detection sites, and low throughput , to achieve the effect of making up for the limitation of sequencing read length, high accuracy and large throughput

Inactive Publication Date: 2018-11-02
CHEERLAND BIOTECH CO LTD
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Problems solved by technology

Among them, the advantage of the sanger sequencing method is that it can detect known and unknown mutations in the target region, but its disadvantage is that the throughput is low and it is not suitable for large-scale screening
Chip hybridization and fluorescent quantitative PCR methods have relatively higher throughput, but only known mutations can be detected, and the detection sites are relatively small. During the large-scale screening of thalassemia, some rare mutations may be caused. missed detection

Method used

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  • Library building method for screening large samples of thalassemia based on high-throughput sequencing
  • Library building method for screening large samples of thalassemia based on high-throughput sequencing
  • Library building method for screening large samples of thalassemia based on high-throughput sequencing

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Embodiment

[0071] In this embodiment, the specific primers with the tag sequence (the first 6 bases at the 5' end) shown in Table 1 were used to amplify HBA1, HBA2 and HBB genes, respectively. Among them, for the HBA1 and HBA2 genes, there are 96 pairs of specific primers (seq1 to seq96), which are used for the amplification of 96 samples respectively; for the HBB gene, the amplification is divided into two sections (ie, HBB1, HBB2), each There are 96 pairs of specific primers (seq1 to seq96), which are used for the amplification of 96 samples respectively. For each gene fragment of each sample, use a pair of specific specific primers (for example, HBA1-F and HBA1-R of seq1).

[0072] Table 1

[0073]

[0074]

[0075]

[0076]

[0077]

[0078]

[0079]

[0080]

[0081]

[0082]

[0083]

[0084] (1) The reaction system is as follows in Table 2:

[0085] Table 2

[0086]

[0087] The reaction program was: thermal denaturation at 95°C for 3 min; de...

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Abstract

The invention discloses a library building method for screening large samples of thalassemia based on high-throughput sequencing. The library building method comprises the following steps: respectively amplifying HBA1, HBA2 and HBB genes by using specific primers with tag sequences, wherein the tag sequences are used for distinguishing different samples; mixing amplification products with same genes from different samples and then mixing the mixed amplification products with different genes; purifying the mixed products; incompletely interrupting the purified products; carrying out 5' phosphorylation blunt end repair and 3' end plus A to obtain a DNA segment with 5' phosphorylation and 3' viscous end A; ligating the DNA fragment with a connector containing a unique barcode sequence for distinguishing the library; purifying a ligation product to obtain an upper computer library suitable for the high-throughput sequencing. The method disclosed by the invention has the advantages that 245kinds of HBB gene mutation types and 93 kinds of HBA gene mutation types which are currently known and related to the thalassemia can be covered; meanwhile, novel types in the target area range can also be detected.

Description

technical field [0001] The invention relates to the technical field of thalassemia detection, in particular to a method for building a library based on high-throughput sequencing for screening large samples of thalassemia. Background technique [0002] Thalassemia is a thalassemia in which the synthesis of one or more globin chains in hemoglobin is absent or deficient due to a genetic defect. γ, δ, and β globin form the β gene family, and ζ and α globin form the α gene family; thalassemia is also divided into four types: α type, β type, δβ type, and δ type, among which β and α thalassemias are more common. common. The α-thalassemia-related genes include HBA2 and HBA1, and the β-thalassemia-related genes are HBB; there are as many as 348 types on HBA1, 431 mutation types on HBA2, and 887 mutation types on HBB; Among them, there are 484 mutation types related to thalassemia, including large deletions, point mutations, and deletion duplications. [0003] The occurrence of th...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C40B50/06
CPCC12N15/1093C40B50/06C12Q2563/185C12Q2525/191
Inventor 陈川陈建国张静王瑢杨传春张文勇
Owner CHEERLAND BIOTECH CO LTD
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