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常用法医DNA提取方案对单链DNA/双链DNA比例及DNA完整性的影响。

The effect of commonly employed forensic DNA extraction protocols on ssDNA/dsDNA proportion and DNA integrity.

作者信息

Stoljarova-Bibb Monika, Sadam Maarja, Erg Silja, Väli Marika

机构信息

Estonian Forensic Science Institute, Tallinn, Estonia.

Estonian Forensic Science Institute, Tallinn, Estonia.

出版信息

Forensic Sci Int Genet. 2025 Mar;76:103210. doi: 10.1016/j.fsigen.2024.103210. Epub 2024 Dec 17.

Abstract

The utilisation of massively parallel sequencing (MPS) in forensic DNA analysis is on the rise, driven by the expansion of targeted MPS panels in the market and the introduction of forensic investigative genetic genealogy. The MPS library preparation process, integral to both whole-genome sequencing (WGS) and targeted MPS panel data generation, is largely based on converting double-stranded DNA (dsDNA) into sequencing libraries. In the current study, we examined the effect of seven routinely used forensic DNA extraction methods on the strandedness (single-stranded or double-stranded) and the fragment size of the DNA extracted from buccal swab, blood, bone and tooth samples. Our findings reveal a variation in the proportion of dsDNA and single-stranded DNA (ssDNA), with the phenol-chloroform and silica column-based extraction methods tested predominantly yielding dsDNA, while the tested Chelex and magnetic bead-based extraction methods predominantly yielded ssDNA. Additionally, fragment size analysis showed that high molecular weight dsDNA was recovered from buccal swab samples with all of the extraction methods except Chelex, which yielded relatively short dsDNA fragments. DNA extracted from tooth samples with tested magnetic bead-based extraction methods resulted in longer dsDNA fragments compared to the silica column-based extraction protocol.

摘要

在法医DNA分析中,大规模平行测序(MPS)的应用正在增加,这是由市场上靶向MPS面板的扩展以及法医调查遗传谱系学的引入所推动的。MPS文库制备过程是全基因组测序(WGS)和靶向MPS面板数据生成所不可或缺的,主要基于将双链DNA(dsDNA)转化为测序文库。在本研究中,我们检测了七种常用的法医DNA提取方法对从口腔拭子、血液、骨骼和牙齿样本中提取的DNA的链性(单链或双链)和片段大小的影响。我们的研究结果显示,dsDNA和单链DNA(ssDNA)的比例存在差异,测试的酚-氯仿法和基于硅胶柱的提取方法主要产生dsDNA,而测试的Chelex法和基于磁珠的提取方法主要产生ssDNA。此外,片段大小分析表明,除Chelex法产生相对较短的dsDNA片段外,所有提取方法均能从口腔拭子样本中回收高分子量dsDNA。与基于硅胶柱的提取方案相比,用测试的基于磁珠的提取方法从牙齿样本中提取的DNA产生的dsDNA片段更长。

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