Noninvasive antepartum fetal beta-thalassemia gene mutation detection library building method, detection method and kit
A library construction and thalassemia technology, applied in chemical libraries, biochemical equipment and methods, library creation, etc., can solve the problem of missing homozygous types, low plasma DNA content, and the inability to further determine the existence of maternal mutations, etc. problem, to achieve the effect of improving specificity
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[0089] 1. For β-thalassemia gene mutation sites -90(C>T), -31(A>C), -30(T>C), -29(A>G), -28(A>G / C ), 5'UTR Cap+1(A>C), Initiation codon(ATG>AGG), CD14–15(+G), CD17(AAG>TAG), CD27 / 28(+C), CD31(–C) , CD37(TGG>TAG), CD41–42(–CTTT), CD43(GAG>TAG), CD71–72(+A / T), CD26(GAG>AAG), IVS–I–1(G>T) , IVS–I–5(G>C), IVS–II–654(C>T) designed synthetic primers:
[0090] The upstream primer and downstream primer are located on the left and right of the detection point, respectively. The 3' end of specific primer 1 and the 5' end of specific primer 2 on the same side overlap by 10-15 bases. The 5' end of specific primer 1 was modified with biotin. The 5' end of specific primer 2 contains adapter sequences for high-throughput sequencing libraries. Specifically, the primer sequences are shown in Table 1.
[0091] Table 1
[0092]
[0093]
[0094]
[0095] 2. Linker sequence with specific tag sequence and sample tag sequence (index):
[0096] ADT-F:
[0097] CAAGCAGAAGACGGCATACGAG...
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