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带尾双链DNA是Rad51蛋白介导的同源配对的首选底物。

Tailed duplex DNA is the preferred substrate for Rad51 protein-mediated homologous pairing.

作者信息

Mazin A V, Zaitseva E, Sung P, Kowalczykowski S C

机构信息

Division of Biological Sciences, Sections of Microbiology, University of California, Davis, CA 95616-8665, USA.

出版信息

EMBO J. 2000 Mar 1;19(5):1148-56. doi: 10.1093/emboj/19.5.1148.

Abstract

The repair of potentially lethal DNA double-stranded breaks (DSBs) by homologous recombination requires processing of the broken DNA into a resected DNA duplex with a protruding 3'-single-stranded DNA (ssDNA) tail. Accordingly, the canonical models for DSB repair require invasion of an intact homologous DNA template by the 3'-end of the ssDNA, a characteristic that the bacterial pairing protein RecA possesses. Unexpectedly, we find that for the eukaryotic homolog, Rad51 protein, the 5'-end of ssDNA is more invasive than the 3'-end. This pairing bias is unaffected by Rad52, Rad54 or Rad55-57 proteins. However, further investigation reveals that, in contrast to RecA protein, the preferred DNA substrate for Rad51 protein is not ssDNA but rather dsDNA with ssDNA tails. This important distinction permits the Rad51 proteins to promote DNA strand invasion using either 3'- or 5'-ends with similar efficiency.

摘要

通过同源重组修复潜在致死性DNA双链断裂(DSB)需要将断裂的DNA加工成具有突出3'单链DNA(ssDNA)尾巴的切除DNA双链体。因此,DSB修复的经典模型要求ssDNA的3'端侵入完整的同源DNA模板,这是细菌配对蛋白RecA所具有的特征。出乎意料的是,我们发现对于真核生物同源物Rad51蛋白,ssDNA的5'端比3'端更具侵入性。这种配对偏好不受Rad52、Rad54或Rad55 - 57蛋白的影响。然而,进一步研究表明,与RecA蛋白不同,Rad51蛋白的首选DNA底物不是ssDNA,而是带有ssDNA尾巴的dsDNA。这一重要区别使得Rad51蛋白能够以相似的效率使用3'端或5'端促进DNA链侵入。

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