ABO血型系统
基因分型
生物
单倍型
遗传学
打字
等位基因
外显子
DNA测序
聚合酶链反应
编码区
基因
基因型
作者
Z. X. Wang,Yushuang Chu,Yanlin Xiao,Maohong Bian
摘要
Abstract Background and Objectives Recently, third‐generation long‐read sequencing technology has been increasingly applied to the detection of various blood group systems. Because of its long read length and use of single‐molecule sequencing, it is capable of obtaining the sequences of blood group genes in their entirety as well as of distinguishing haplotypes. Therefore, here, we collected ABO blood group samples that were difficult to classify serologically and analysed the sequences of the coding regions of the ABO genes as well as the sequences upstream and downstream of the coding regions. Materials and Methods Samples with ABO antigen typing and reverse serum typing discrepancies were screened in a total of 21 patients. All samples were subjected to serological testing and preliminary ABO genotyping (polymerase chain reaction with sequence‐specific primers [PCR‐SSP]), followed by single‐molecule real‐time (SMRT) sequencing to obtain complete ABO gene sequences. PCR sequence‐based typing (PCR‐SBT) was performed to validate the results. Results Of the 21 samples, 15 had common ABO types, and 6 had rare ABO subtypes. One new allele, ABO*B.NEW (c.861C>T) , and one allelic base recombination event was identified. Forty‐two haplotype sequences were obtained via SMRT sequencing with intronic single‐nucleotide variants (SNVs) specific to the ABO allele, and all of the exon region sequences were consistent with the PCR‐SBT results. Conclusion SMRT sequencing is capable of accurately obtaining complete ABO gene sequences, distinguishing haplotypes and identifying allelic recombination.
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