利用 Illumina 的 ForenSeq 系统对福尔马林固定骸骨样本进行法医 STR 和 SNP 基因分型。

IF 3 3区 生物学 Q2 BIOCHEMICAL RESEARCH METHODS
Tingting Yang, Linlin Gao, Jiarong Zhang, Wei Xie, Wenjing Hu, Jiangwei Yan
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引用次数: 0

摘要

福尔马林固定剂在法医学中被广泛用于保存组织。然而,从福尔马林固定样本中提取高质量的基因组 DNA 却极具挑战性。使用毛细管电泳(CE)进行法医 DNA 分型的传统短串联重复(STR)分析经常失败。大规模平行测序(MPS)可在一次测试中处理许多样本和数千个遗传标记,通常是单核苷酸多态性(SNP)和 STR。因此,它可用于评估高度变质的法医证据。使用 MPS 对福尔马林固定骨骼进行 STR 和 SNPs 基因分型的有效性研究很少。本研究在 Illumina MiSeq FGX 平台上使用 ForenSeq DNA Signature Prep Kit 对来自 5 个个体的 55 个不同福尔马林固定时间(5-75 天)的骨骼样本进行了检测和测序。结果表明,随着福尔马林固定时间的延长,STR 和 SNP 的检出率逐渐降低。固定 75 天后,STR 和 SNP 的平均检出率分别为 4% 和 10%。个体识别 SNPs(iiSNPs)的累积鉴别力(CDP)在第 45 天时大于 0.9999。然而,在第 22 天,STR 的 CDP 为 0.9930。6 个 STR(D1S1656、PentaE、D22S1045、PentaD、DX8378 和 DX10103)和 5 个 SNP(rs2920816、rs354439、rs1736442、rs338882 和 rs1031825)的检出率较低。总之,从福尔马林固定的骸骨中提取的 DNA 会随着时间的推移迅速分解,而 MPS 技术是检测此类样本中法医遗传标记的有用工具。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Forensic STR and SNP Genotyping of Formalin-Fixed Skeleton Samples With Illumina's ForenSeq System

Formalin fixatives are widely used in forensics to preserve tissues. However, extracting high-quality genomic DNA from formalin-fixed samples is challenging. Traditional short tandem repeat (STR) analysis using capillary electrophoresis (CE) for forensic DNA typing frequently results in failure. Massively parallel sequencing (MPS) can handle many samples and thousands of genetic markers, usually single-nucleotide polymorphisms (SNPs) and STRs, in a single test. Thus, it is useful for assessing highly deteriorated forensic evidence. Few studies have examined the effectiveness of STRs and SNPs genotyping of formalin-fixed skeletons using MPS. In this study, 55 skeletal samples from 5 individuals that were treated under different formalin fixation times (5–75 days) were examined and sequenced using the ForenSeq DNA Signature Prep Kit on the Illumina MiSeq FGX platform. The results showed that as the duration of formalin fixation increased, the detection rates of STRs and SNPs gradually decreased. After 75 days of fixation, the average detection rates for STRs and SNPs were 4% and 10%, respectively. The cumulative discrimination power (CDP) of individual identification SNPs (iiSNPs) was >0.9999 on the 45th day. However, the CDP of STRs was 0.9930 on the 22nd day. Low detection rates were observed for six STRs (D1S1656, PentaE, D22S1045, PentaD, DX8378 and DX10103) and five SNPs (rs2920816, rs354439, rs1736442, rs338882 and rs1031825). In conclusion, DNA extracted from formalin-fixed skeletons decomposes rapidly over time, and MPS technology can be a useful tool for detecting forensic genetic markers in such samples.

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来源期刊
ELECTROPHORESIS
ELECTROPHORESIS 生物-分析化学
CiteScore
6.30
自引率
13.80%
发文量
244
审稿时长
1.9 months
期刊介绍: ELECTROPHORESIS is an international journal that publishes original manuscripts on all aspects of electrophoresis, and liquid phase separations (e.g., HPLC, micro- and nano-LC, UHPLC, micro- and nano-fluidics, liquid-phase micro-extractions, etc.). Topics include new or improved analytical and preparative methods, sample preparation, development of theory, and innovative applications of electrophoretic and liquid phase separations methods in the study of nucleic acids, proteins, carbohydrates natural products, pharmaceuticals, food analysis, environmental species and other compounds of importance to the life sciences. Papers in the areas of microfluidics and proteomics, which are not limited to electrophoresis-based methods, will also be accepted for publication. Contributions focused on hyphenated and omics techniques are also of interest. Proteomics is within the scope, if related to its fundamentals and new technical approaches. Proteomics applications are only considered in particular cases. Papers describing the application of standard electrophoretic methods will not be considered. Papers on nanoanalysis intended for publication in ELECTROPHORESIS should focus on one or more of the following topics: • Nanoscale electrokinetics and phenomena related to electric double layer and/or confinement in nano-sized geometry • Single cell and subcellular analysis • Nanosensors and ultrasensitive detection aspects (e.g., involving quantum dots, "nanoelectrodes" or nanospray MS) • Nanoscale/nanopore DNA sequencing (next generation sequencing) • Micro- and nanoscale sample preparation • Nanoparticles and cells analyses by dielectrophoresis • Separation-based analysis using nanoparticles, nanotubes and nanowires.
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