由 201 个遗传标记组成的降解样本 DNA 分型小组:开发与验证。

Q3 Medicine 遗传 Pub Date : 2024-04-20 DOI:10.16288/j.yczz.23-253
Wei Han, Qing-Zhen Zhang, Jing Yang, Zhe Zhou
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引用次数: 0

摘要

近年来,随着复杂法医案件的增多,将短串联重复序列(STRs)、单核苷酸多态性(SNPs)、插入/缺失多态性(InDels)和微位型(MHs)等不同类型的遗传标记结合起来以提供更多的遗传信息显得更为重要。本研究选择了 201 个遗传标记,包括 24 个常染色体 STR(A-STR)、24 个 Y 染色体 STR(Y-STR)、110 个 A-SNP、24 个 Y-SNP、9 个 A-InDels、1 个 Y-InDel、8 个 MH 和 Amelogenin,建立了下一代测序(NGS)检测系统 HID_AM Panel v1.0。根据 DNA 分析方法科学工作组(SWGDAM)的验证指南,对该系统的重复性、准确性、灵敏度、对降解样本的适用性、物种特异性和抑制剂抗性进行了评估。该系统对 48 种 STR 和安美尔基因的分型结果与毛细管电泳的结果完全一致。使用 ForenSeq™ DNA Signature Prep Kit 的 FGx 测序仪同时确认了该系统对 79 个 SNP 的准确检测。输入不少于 200 pg 的 DNA 即可获得完整的等位基因分型结果。当模拟降解样本的降解指数大于 15.87 时,该系统的检测成功率明显高于 GlobalFiler™ 试剂盒。当扩增系统中赤血素浓度≤40 µmol/L、靛蓝浓度≤2 mmol/L或腐植酸浓度≤15 ng/µL时,扩增未受到明显抑制。该系统几乎不能扩增鸭、鼠、牛、兔和鸡的 DNA 提取物。该检测板常规样本的 STR 检测率为 99.74%,所有 SNPs、InDels 和 MHs 均检测成功。综上所述,我们建立了一个包括 201 个遗传标记的 NGS 个体分型面板,该面板具有较高的准确性、灵敏度、物种特异性和抗抑制剂性,适用于降解样本的个体鉴定。
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A DNA typing panel of 201 genetic markers for degraded samples: development and validation.

With the increasing number of complex forensic cases in recent years, it's more important to combine the different types of genetic markers such as short tandem repeats (STRs), single nucleotide polymorphisms (SNPs), insertion/deletion polymorphisms (InDels), and microhaplotypes (MHs) to provide more genetic information. In this study, we selected totally 201 genetic markers, including 24 autosomes STRs (A-STRs), 24 Y chromosome STRs (Y-STRs), 110 A-SNPs, 24 Y-SNPs, 9 A-InDels, 1 Y-InDel, 8 MHs, and Amelogenin to establish the HID_AM Panel v1.0, a Next-Generation Sequencing (NGS) detection system. According to the validation guidelines of the Scientific Working Group on DNA Analysis Methods (SWGDAM), the repeatability, accuracy, sensitivity, suitability for degraded samples, species specificity, and inhibitor resistance of this system were assessed. The typing results on 48 STRs and Amelogenin of this system were completely consistent with those obtained using capillary electrophoresis. This system accurately detected 79 SNPs as parallelly confirmed by a FGx sequencer with the ForenSeq™ DNA Signature Prep Kit. Complete allele typing results could be obtained with a DNA input of no less than 200 pg. The detection success rate of this system was significantly higher than that of the GlobalFiler™ kit when the degradation index of mock degraded sample was greater than 15.87. When the concentration of hematin in the amplification system was ≤40 µmol/L, indigo blue was ≤2 mmol/L, or humic acid was ≤15 ng/µL, amplification was not significantly inhibited. The system barely amplified the DNA extract from duck, mouse, cow, rabbit, and chick. The detection rate of STRs on routine samples of this panel is 99.74%, while all the SNPs, InDels, and MHs were successfully detected. In summary, we setup a NGS individual typing panel including 201 genetic markers with the high accuracy, sensitivity, species specificity, and inhibitors resistance, which is applicable for individual identification of degraded samples.

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来源期刊
遗传
遗传 Medicine-Medicine (all)
CiteScore
2.50
自引率
0.00%
发文量
6699
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