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
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[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
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[0084] (1) The reaction system is as follows in Table 2:
[0085] Table 2
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[0087] The reaction program was: thermal denaturation at 95°C for 3 min; de...
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