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一种用于定量分析雄配子和雌配子中各个重组热点处交叉和非交叉分子事件的检测方法。

A quantitative assay for crossover and noncrossover molecular events at individual recombination hotspots in both male and female gametes.

作者信息

Ng Siemon H, Parvanov Emil, Petkov Petko M, Paigen Kenneth

机构信息

Center for Genome Dynamics, The Jackson Laboratory, Bar Harbor, ME 04609, USA.

出版信息

Genomics. 2008 Oct;92(4):204-9. doi: 10.1016/j.ygeno.2008.06.008. Epub 2008 Aug 12.

Abstract

Meiotic recombination is a fundamental process in all eukaryotes. Among organisms in which recombination initiates prior to synapsis, recombination preferentially occurs in short 1-to 2-kb regions, known as recombination hotspots. Among mammals, genotyping sperm DNA has provided a means of monitoring recombination events at specific hotspots in male meiosis. To complement these current techniques, we developed an assay for amplifying all copies of a hotspot from the DNA of male and female germ cells, cloning the products into Escherichia coli, and SNP genotyping the resulting colonies using fluorescence technology. This approach examines the molecular details of crossover and noncrossover events of individual meioses directly at active hotspots while retaining the simplicity of using pooled DNA. Using this technique, we analyzed recombination events at the Hlx1 hotspot located on mouse chromosome 1, finding that the results agree well with a prior genetic characterization of 3026 male and 3002 female meioses.

摘要

减数分裂重组是所有真核生物中的一个基本过程。在那些重组先于联会起始的生物体中,重组优先发生在短的1至2千碱基区域,即所谓的重组热点。在哺乳动物中,对精子DNA进行基因分型提供了一种监测雄性减数分裂中特定热点处重组事件的方法。为了补充这些现有技术,我们开发了一种检测方法,用于从雄性和雌性生殖细胞的DNA中扩增热点的所有拷贝,将产物克隆到大肠杆菌中,并使用荧光技术对所得菌落进行单核苷酸多态性(SNP)基因分型。这种方法直接在活跃热点处检查单个减数分裂的交叉和非交叉事件的分子细节,同时保留了使用混合DNA的简便性。利用这项技术,我们分析了位于小鼠1号染色体上的Hlx1热点处的重组事件,发现结果与之前对3026个雄性和3002个雌性减数分裂的遗传特征分析结果非常吻合。

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