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小鼠基因组中精细的重组率和热点图谱。

Fine-scale maps of recombination rates and hotspots in the mouse genome.

机构信息

Department of Statistics, The Hebrew University of Jerusalem, Jerusalem 91905, Israel.

出版信息

Genetics. 2012 Jul;191(3):757-64. doi: 10.1534/genetics.112.141036. Epub 2012 May 4.

Abstract

Recombination events are not uniformly distributed and often cluster in narrow regions known as recombination hotspots. Several studies using different approaches have dramatically advanced our understanding of recombination hotspot regulation. Population genetic data have been used to map and quantify hotspots in the human genome. Genetic variation in recombination rates and hotspots usage have been explored in human pedigrees, mouse intercrosses, and by sperm typing. These studies pointed to the central role of the PRDM9 gene in hotspot modulation. In this study, we used single nucleotide polymorphisms (SNPs) from whole-genome resequencing and genotyping studies of mouse inbred strains to estimate recombination rates across the mouse genome and identified 47,068 historical hotspots--an average of over 2477 per chromosome. We show by simulation that inbred mouse strains can be used to identify positions of historical hotspots. Recombination hotspots were found to be enriched for the predicted binding sequences for different alleles of the PRDM9 protein. Recombination rates were on average lower near transcription start sites (TSS). Comparing the inferred historical recombination hotspots with the recent genome-wide mapping of double-strand breaks (DSBs) in mouse sperm revealed a significant overlap, especially toward the telomeres. Our results suggest that inbred strains can be used to characterize and study the dynamics of historical recombination hotspots. They also strengthen previous findings on mouse recombination hotspots, and specifically the impact of sequence variants in Prdm9.

摘要

重组事件并非均匀分布,而是经常聚集在称为重组热点的狭窄区域。使用不同方法的几项研究极大地提高了我们对重组热点调控的理解。群体遗传数据已被用于绘制和量化人类基因组中的热点。在人类家系、小鼠杂交和精子分型中,研究了重组率和热点使用的遗传变异。这些研究指出 PRDM9 基因在热点调节中的核心作用。在这项研究中,我们使用全基因组重测序和小鼠近交系的基因分型研究中的单核苷酸多态性 (SNP) 来估计整个小鼠基因组中的重组率,并确定了 47,068 个历史热点——平均每个染色体超过 2477 个。我们通过模拟表明,近交系小鼠可以用于识别历史热点的位置。发现重组热点富含不同 PRDM9 蛋白等位基因的预测结合序列。重组率在转录起始位点 (TSS) 附近平均较低。将推断的历史重组热点与最近在小鼠精子中全基因组范围内的双链断裂 (DSB) 作图进行比较时,发现存在显著重叠,尤其是在端粒附近。我们的结果表明,近交系可以用于表征和研究历史重组热点的动态。它们还加强了先前关于小鼠重组热点的发现,特别是 Prdm9 中序列变异的影响。

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