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DIP-STR: Highly Sensitive Markers for the Analysis of Unbalanced Genomic Mixtures.

机译:DIP-STR:用于非平衡基因组混合物分析的高灵敏度标记。

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摘要

Samples containing highly unbalanced DNA mixtures from two individuals commonly occur both in forensic mixed stains and in peripheral blood DNA microchimerism induced by pregnancy or following organ transplant. Because of PCR amplification bias, the genetic identification of a DNA that contributes trace amounts to a mixed sample represents a tremendous challenge. This means that standard genetic markers, namely microsatellites, also referred as short tandem repeats (STR), and single-nucleotide polymorphism (SNP) have limited power in addressing common questions of forensic and medical genetics. To address this issue, we developed a molecular marker, named DIP-STR that relies on pairing deletion-insertion polymorphisms (DIP) with STR. This novel analytical approach allows for the unambiguous genotyping of a minor component in the presence of a major component, where DIP-STR genotypes of the minor were successfully procured at ratios up to 1:1,000. The compound nature of this marker generates a high level of polymorphism that is suitable for identity testing. Here, we demonstrate the power of the DIP-STR approach on an initial set of nine markers surveyed in a Swiss population. Finally, we discuss the limitations and potential applications of our new system including preliminary tests on clinical samples and estimates of their performance on simulated DNA mixtures.
机译:包含两个个体的高度不平衡DNA混合物的样品通常出现在法医混合染色和妊娠或器官移植后诱导的外周血DNA微嵌合中。由于PCR扩增的偏见,对痕量混合样品中的DNA进行遗传鉴定面临着巨大的挑战。这意味着标准遗传标记,即微卫星,也称为短串联重复序列(STR)和单核苷酸多态性(SNP),在解决法医和医学遗传学的常见问题方面的作用有限。为了解决这个问题,我们开发了一种分子标记,称为DIP-STR,它依赖于STR的缺失插入多态性(DIP)。这种新颖的分析方法可以在存在主要成分的情况下对次要成分进行明确的基因分型,其中成功以1:1:1,000的比例成功获得了次要成分的DIP-STR基因型。此标记的复合性质会产生高水平的多态性,适用于身份测试。在这里,我们展示了DIP-STR方法在瑞士人口调查的最初九个标记集上的作用。最后,我们讨论了我们新系统的局限性和潜在应用,包括对临床样品的初步测试以及对模拟DNA混合物的性能评估。

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