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Rad52在双链断裂修复中促进第二末端DNA捕获,以形成互补稳定的接头分子。

Rad52 promotes second-end DNA capture in double-stranded break repair to form complement-stabilized joint molecules.

作者信息

Nimonkar Amitabh V, Sica R Alejandro, Kowalczykowski Stephen C

机构信息

Department of Microbiology, University of California, Davis, CA 95616-8665, USA.

出版信息

Proc Natl Acad Sci U S A. 2009 Mar 3;106(9):3077-82. doi: 10.1073/pnas.0813247106. Epub 2009 Feb 9.

Abstract

Saccharomyces cerevisiae Rad52 performs multiple functions during the recombinational repair of double-stranded DNA (dsDNA) breaks (DSBs). It mediates assembly of Rad51 onto single-stranded DNA (ssDNA) that is complexed with replication protein A (RPA); the resulting nucleoprotein filament pairs with homologous dsDNA to form joint molecules. Rad52 also catalyzes the annealing of complementary strands of ssDNA, even when they are complexed with RPA. Both Rad51 and Rad52 can be envisioned to promote "second-end capture," a step that pairs the ssDNA generated by processing of the second end of a DSB to the joint molecule formed by invasion of the target dsDNA by the first processed end. Here, we show that Rad52 promotes annealing of complementary ssDNA that is complexed with RPA to the displaced strand of a joint molecule, to form a complement-stabilized joint molecule. RecO, a prokaryotic homolog of Rad52, cannot form complement-stabilized joint molecules with RPA-ssDNA complexes, nor can Rad52 promote second-end capture when the ssDNA is bound with either human RPA or the prokaryotic ssDNA-binding protein, SSB, indicating a species-specific process. We conclude that Rad52 participates in second-end capture by annealing a resected DNA break, complexed with RPA, to the joint molecule product of single-end invasion event. These studies support a role for Rad52-promoted annealing in the formation of Holliday junctions in DSB repair.

摘要

酿酒酵母Rad52在双链DNA(dsDNA)断裂(DSB)的重组修复过程中发挥多种功能。它介导Rad51组装到与复制蛋白A(RPA)复合的单链DNA(ssDNA)上;由此产生的核蛋白丝与同源dsDNA配对形成连接分子。Rad52还催化ssDNA互补链的退火,即使它们与RPA复合。可以设想Rad51和Rad52都能促进“第二末端捕获”,这一步骤将由DSB第二末端加工产生的ssDNA与由第一个加工末端侵入靶dsDNA形成的连接分子配对。在这里,我们表明Rad52促进与RPA复合的互补ssDNA与连接分子的置换链退火,形成互补稳定的连接分子。RecO是Rad52的原核同源物,不能与RPA-ssDNA复合物形成互补稳定的连接分子,当ssDNA与人RPA或原核ssDNA结合蛋白SSB结合时,Rad52也不能促进第二末端捕获,这表明这是一个物种特异性过程。我们得出结论,Rad52通过将与RPA复合的切除DNA断裂退火到单末端侵入事件的连接分子产物上,参与第二末端捕获。这些研究支持Rad52促进的退火在DSB修复中Holliday连接形成中的作用。

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