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SNP discovery by mismatch-targeting of Mu transposition

机译:通过错位靶向Mu换位发现SNP

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摘要

Single nucleotide polymorphisms (SNPs) represent a valuable resource for the mapping of human disease genes and induced mutations in model organisms. SNPs may become the markers of choice also for population ecology and evolutionary studies, but their isolation for non-model organisms with unsequenced genomes is often difficult. Here, we describe a rapid and cost-effective strategy to isolate SNPs that exploits the property of the bacteriophage Mu transposition machinery to target mismatched DNA sites and thereby to effectively detect polymorphic loci. To demonstrate the methodology, we isolated 164 SNPs from the unsequenced genome of the Glanville fritillary butterfly (Melitaea cinxia), a much-studied species in population biology, and we validated 24 of them. The strategy involves standard molecular biology techniques as well as undemanding MuA transposase-catalyzed in vitro transposition reactions, and it is applicable to any organism.
机译:单核苷酸多态性(SNP)代表了宝贵的资源,可用于绘制人类疾病基因和模型生物中的诱发突变。 SNP也可能成为种群生态学和进化研究的选择标记,但是要分离具有未测序基因组的非模式生物通常很难。在这里,我们描述了一种分离SNP的快速且经济高效的策略,该策略利用噬菌体Mu转座机制的特性来靶向错配的DNA位点,从而有效地检测多态性基因座。为了证明该方法,我们从未进行测序的Glanville贝母蝴蝶(Melitaea cinxia)的基因组中分离了164个SNP,这是在种群生物学中被广泛研究的物种,我们验证了其中的24个。该策略涉及标准分子生物学技术以及不需要的MuA转座酶催化的体外转座反应,并且适用于任何生物。

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