微卫星
大规模并行测序
STR复用系统
多路复用
遗传学
单核苷酸多态性
放大器
计算生物学
SNP公司
生物
STR分析
基因型
人口
DNA测序
计算机科学
DNA
聚合酶链反应
医学
基因
等位基因
环境卫生
作者
Ruiyang Tao,Shouyu Wang,Anqi Chen,Ruocheng Xia,Xiaochun Zhang,Qi Yang,Yiling Qu,Suhua Zhang,Chengtao Li
标识
DOI:10.1016/j.fsigen.2021.102490
摘要
Massively parallel sequencing (MPS), or next generation sequencing (NGS), is a promising methodology for the detection of short tandem repeats (STRs) and single nucleotide polymorphisms (SNPs) in forensic genetics. Here, the prototype SifaMPS Panel is designed to simultaneously target 87 STRs and 294 SNPs with forensic interest in a single multiplex in conjunction with the TruSeq™ Custom Amplicon workflow and MiSeq FGx™ System. Two in-house python scripts are adopted for the fastq-to-genotype interpretation of MPS data concerning STR and SNP, respectively. In the present study, by sequencing 50 Chinese Hans and many other DNA samples involved in validation studies, system parameters including the depth of coverage (DoC), heterozygote balance (Hb) and sequence coverage ratios (SCRs), as well as different forensic parameters of STRs and SNPs in a population study, were calculated to evaluate the overall performance of this new panel and its practicality in forensic application. In general, except for two STRs (DYS505 and DYS449) and one SNP (rs4288409) that performed poorly, the other 85 STRs and 293 SNPs in our panel had good performance that could strengthen efficiency for human identification and paternity testing. In addition, discordant STR genotype results between those generated from capillary electrophoresis (CE) and from the MPS platform were clearly illustrated, and these results could be a useful reference for applying these particular non-CODIS STRs in forensic practice.
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