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Approaches for identifying multiple-SNP haplotype blocks for use in human identification

机译:识别用于人类识别的多个SNP单倍型模块的方法

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Single nucleotide polymorphism (SNP) discrimination effectiveness is low due to the bi-allelic nature of SNPs, and large numbers of loci must be analyzed for human identification in forensic casework. To resolve these issues, the authors support the use of multiple SNP haplotypes that will generate many haplotypes based on the combination of SNP alleles. First, 27 regions were selected from the JSNP database (http://snp.ims.u-tokyo.ac.jp) according to the following criteria: (1) 3 or more SNP loci within 100 bp; (2) on-intron or out-of-gene location; and (3) frequency of more than 40% for each SNP allele. PCR amplification and high-resolution melting curve (HRM) analysis were then carried out for all selected regions to determine variation in the haplotypes of each. HRM analysis indicated that 7 regions (1q25, 1q42.2, 3p24, 10p13, 11p15.1, 14q12-q13, and 20q12) containing 3 SNP loci had more than 2 haplotypes. The frequencies of the haplotypes for each region were observed via direct sequencing of more than 100 individuals. Not only haplotyping increases the effectiveness of individual identification but also the analysis region is shorter than in common short tandem repeat analysis, representing a further advantage for fragmented DNA samples in SNP typing. (C) 2015 Elsevier Ireland Ltd. All rights reserved.
机译:由于单核苷酸多态性(SNP)的双等位基因性质,其单核苷酸多态性(SNP)判别效率低,在法医案件中必须分析大量基因座以供人类识别。为了解决这些问题,作者支持使用多个SNP单倍型,这些单倍型将根据SNP等位基因的组合生成许多单倍型。首先,根据以下标准从JSNP数据库(http://snp.ims.u-tokyo.ac.jp)中选择27个区域:(1)100 bp内的3个或更多SNP位点; (2)内含子或基因外的位置; (3)每个SNP等位基因的频率超过40%。然后对所有选定区域进行PCR扩增和高分辨率熔解曲线(HRM)分析,以确定每个单倍型的变异。 HRM分析表明,包含3个SNP位点的7个区域(1q25、1q42.2、3p24、10p13、11p15.1、14q12-q13和20q12)具有2个以上的单倍型。通过直接测序超过100个个体,观察到每个区域的单倍型频率。单倍型不仅提高了个体识别的效率,而且与普通的短串联重复分析相比,分析区域更短,这代表了SNP分型中片段化DNA样品的进一步优势。 (C)2015 Elsevier Ireland Ltd.保留所有权利。

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