Phillips Christopher, García-Magariños Manuel, Salas Antonio, Carracedo Angel, Lareu Maria Victoria
Forensic Genetics Unit, Institute of Legal Medicine, University of Santiago de Compostela, Santiago de Compostela, Galicia, Galicia, Spain.
Transfus Med Hemother. 2012 Jun;39(3):202-210. doi: 10.1159/000338857. Epub 2012 May 12.
Genetic tests for kinship testing routinely reach likelihoods that provide virtual proof of the claimed relationship by typing microsatellites-commonly consisting of 12-15 standard forensic short tandem repeats (STRs). Single nucleotide polymorphisms (SNPs) have also been applied to kinship testing but these binary markers are required in greater numbers than multiple-allele STRs. However SNPs offer certain advantageous characteristics not found in STRs, including, much higher mutational stability, good performance typing highly degraded DNA, and the ability to be readily up-scaled to very high marker numbers reaching over a million loci. This article outlines kinship testing applications where SNPs markedly improve the genetic data obtained. In particular we explore the minimum number of SNPs that will be required to confirm pairwise relationship claims in deficient pedigrees that typify missing persons' identification or war grave investigations where commonly few surviving relatives are available for comparison and the DNA is highly degraded. METHODS: We describe the application of SNPs alongside STRs when incomplete profiles or allelic instability in STRs create ambiguous results, we review the use of high density SNP arrays when the relationship claim is very distant, and we outline simulations of kinship analyses with STRs supplemented with SNPs in order to estimate the practical limit of pairwise relationships that can be differentiated from random unrelated pairs from the same population. RESULTS: The minimum number of SNPs for robust statistical inference of parent-offspring relationships through to those of second cousins (S-3-3) is estimated for both simple, single multiplex SNP sets and for subsets of million-SNP arrays. CONCLUSIONS: There is considerable scope for resolving ambiguous STR results and for improving the statistical power of kinship analysis by adding small-scale SNP sets but where the pedigree is deficient the pairwise relationships must be relatively close. For more distant relationships it is possible to reduce chip-based SNP arrays from the million+ markers down to ∼7,000. However, such numbers indicate that current genotyping approaches will not be able to deliver sufficient data to resolve distant pairwise relationships from the limited DNA typical of the most challenging identification cases.
亲缘关系检测的基因测试通常通过对微卫星进行分型来得出能为所声称的亲属关系提供实质证据的似然率,微卫星通常由12 - 15个标准法医短串联重复序列(STR)组成。单核苷酸多态性(SNP)也已应用于亲缘关系检测,但这些二元标记物所需数量比多等位基因STR更多。然而,SNP具有一些STR所没有的优势特性,包括更高的突变稳定性、对高度降解DNA进行分型的良好性能,以及能够轻松扩展到超过一百万个位点的非常高的标记数量。本文概述了SNP能显著改善所获基因数据的亲缘关系检测应用。特别是,我们探讨了在典型的失踪人员身份识别或战争坟墓调查等不完整谱系中确认成对亲属关系声明所需的最少SNP数量,在这些情况下,通常很少有在世亲属可供比较且DNA高度降解。
我们描述了在STR的不完整图谱或等位基因不稳定性产生模糊结果时SNP与STR一起的应用,我们回顾了在亲属关系声明非常疏远时高密度SNP阵列的使用,并且我们概述了用补充有SNP的STR进行亲缘关系分析的模拟,以便估计可以与来自同一人群的随机无关对区分开的成对关系的实际限度。
对于简单的单重SNP集和百万SNP阵列的子集,估计了通过二级表亲(S - 3 - 3)直至亲子关系进行稳健统计推断所需的最少SNP数量。
通过添加小规模SNP集来解决模糊的STR结果并提高亲缘关系分析的统计能力有相当大的空间,但在谱系不完整的情况下,成对关系必须相对密切。对于更远的关系,有可能将基于芯片的SNP阵列从超过一百万个标记减少到约7000个。然而,这样的数量表明当前的基因分型方法将无法提供足够的数据来从最具挑战性的身份识别案例中典型的有限DNA中解析出遥远的成对关系。
