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Expanding beyond the current core STR loci: An exploration of 73 STR markers with increased diversity for enhanced DNA mixture deconvolution

机译:超出当前核心STR基因座的扩展:对增强DNA混合卷积的增强的多样性增加了73 str标记的探索

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Current approaches to mixture deconvolution of complex biological samples at times do not have the capability to resolve component contributors in DNA evidence. Additional short tandem repeat (STR) loci were sought that may improve the forensic genetic analysis of mixtures. This study presents exploratory data of a multiplex comprised of 73 highly polymorphic STRs (referred herein as the 73Plex) that were selected because of their high diversity due to sequence variation. These STRs (or a subset of them) may be considered as candidates that may augment current core markers capabilities for DNA mixture deconvolution. Population genetics analyses were performed for each locus using DNA samples from 451 individuals comprising three U.S. populations. Sequence-based heterozygosities ranged from 72% to 98%, where only two loci (D10A97 and D6A7) fell below 80%. Mixture deconvolution capabilities for two-person mixtures were assessed based on complete allele resolution per locus (i.e., four alleles observed) of pairwise mixtures using in silico methods. A subset of 20 highly in- formative loci (referred herein as the 20Plex) from the 73Plex was compared to the 20 CODIS core loci on all population samples with full DNA profiles for both panels (i.e., no locus dropout; n = 443). Based on proportion of loci displaying four alleles, the 20Plex outperformed the CODIS core loci with increases of 82.6% and 89.3% using length-based and sequence-based alleles, respectively. A combination of 17 STR from the 20Plex and 3 CODIS loci gave the highest capacity for resolving allelic components per locus. These data illustrate the increased value of utilizing sequenced-based alleles of additional STR loci. Furthermore, there are a number of candidate STR loci that could notably augment the current core STR loci and enhance mixture interpretation capabilities.
机译:在络合物生物样品混合去卷积的电流方法有时不具有解析DNA证据中的组分贡献的能力。寻求额外的短串联重复(STR)基因座,可以改善混合物的法医遗传分析。该研究提出了由73个高度多态性strs(在本文中称为73plex)的多路复用的探索性数据,因为它们由于序列变异而具有高多样性。这些strs(或它们的子集)可以被认为是可以增强当前核心标记能力的候选者,用于DNA混合卷积卷积。使用来自包含三种U.S.群体的451个个体的DNA样品对每个基因座进行群体遗传分析。基于序列的杂合子范围为72%至98%,其中仅两个基因座(D10A97和D6A7)低于80%。基于使用在硅方法中的成对混合物的每位基因座(即四个等位基因)的完全等位基因分辨率评估双人混合物的混合物去卷积能力。将来自73plex的高度形成的基因座(本文称为20Plect)的子集与所有群体样本的20个Codis核心基因座进行比较,所述群体样本对于两个面板(即,没有基因座丢失; n = 443)。基于显示四个等位基因的基因座的比例,20Plex从基于长度和基于序列的等位基因分别增加了82.6%和89.3%的Codis核心基因座。来自20Plect和3个Codis基因座的17 st的组合具有最高容量,用于解决每个基因座的等位基因组件。这些数据说明利用附加STR基因座的序列基等位基因的增加的值。此外,存在许多候选str基因座,可以尤比增强当前的核心str基因座并增强混合解释能力。

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