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使用亚硫酸氢盐修饰和焦磷酸测序通过组织特异性差异DNA甲基化鉴定精子

Identification of spermatozoa by tissue-specific differential DNA methylation using bisulfite modification and pyrosequencing.

作者信息

Balamurugan Kuppareddi, Bombardi Robin, Duncan George, McCord Bruce

机构信息

School of Criminal Justice, The University of Southern Mississippi, Hattiesburg, MS, USA.

出版信息

Electrophoresis. 2014 Nov;35(21-22):3079-86. doi: 10.1002/elps.201400175. Epub 2014 Jul 28.

DOI:10.1002/elps.201400175
PMID:24913642
Abstract

The focus of this study is to evaluate the application of epigenetic markers as a forensic tool for the determination of semen present in sexual assault cases. A series of genetic loci were screened in order to identify certain epigenetic markers displaying differential methylation that can allow semen to be differentiated from blood, buccal cells, skin epidermis, and vaginal epithelial cells. Of the different loci tested, a panel of six markers, DACT1, USP49, DDX4, Hs_INSL6_03, Hs_ZC3H12D_05, and B_SPTB_03 were identified to contain tissue-specific differential methylation. Samples ranging from 9-21 for each tissue type were collected and subjected to bisulfite modification. The bisulfite modified DNA was amplified by PCR, and analyzed by pyrosequencing to quantitate the level of methylation at each marker. All six markers successfully differentiated semen samples from the other four tissue types analyzed. Sperm DNA was hypomethylated in all but one marker, B_SPTB_03, where this marker showed hypermethylation. Mean methylation percentages for semen samples were statistically significant from mean methylation percentages of the other four tissues studied (p < 0.01). The results of this study demonstrate the applicability of epigenetic markers as a novel tool for determination of spermatozoa and to identify the tissue source of origin of a DNA sample.

摘要

本研究的重点是评估表观遗传标记作为一种法医工具在性侵犯案件中精液鉴定的应用。筛选了一系列基因座,以确定某些显示差异甲基化的表观遗传标记,从而能够将精液与血液、颊细胞、皮肤表皮和阴道上皮细胞区分开来。在测试的不同基因座中,一组六个标记,即DACT1、USP49、DDX4、Hs_INSL6_03、Hs_ZC3H12D_05和B_SPTB_03,被确定含有组织特异性差异甲基化。收集每种组织类型9至21个样本,并进行亚硫酸氢盐修饰。经亚硫酸氢盐修饰的DNA通过PCR扩增,并通过焦磷酸测序进行分析,以定量每个标记的甲基化水平。所有六个标记均成功地将精液样本与其他四种分析的组织类型区分开来。除了一个标记B_SPTB_03外,精子DNA在所有标记中均表现为低甲基化,而该标记显示为高甲基化。精液样本的平均甲基化百分比与所研究的其他四种组织的平均甲基化百分比在统计学上有显著差异(p < 0.01)。本研究结果证明了表观遗传标记作为一种用于确定精子和识别DNA样本组织来源的新型工具的适用性。

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