Mus81、Rhp51(Rad51)和Rqh1形成了S期DNA损伤检查点所需的上位性途径。
Mus81, Rhp51(Rad51), and Rqh1 form an epistatic pathway required for the S-phase DNA damage checkpoint.
作者信息
Willis Nicholas, Rhind Nicholas
机构信息
Department of Biochemistry and Molecular Pharmacology, University of Massachusetts Medical School, Worcester, MA 01605, USA.
出版信息
Mol Biol Cell. 2009 Feb;20(3):819-33. doi: 10.1091/mbc.e08-08-0798. Epub 2008 Nov 26.
Abstract
The S-phase DNA damage checkpoint slows the rate of DNA synthesis in response to damage during replication. In the fission yeast Schizosaccharomyces pombe, Cds1, the S-phase-specific checkpoint effector kinase, is required for checkpoint signaling and replication slowing; upon treatment with the alkylating agent methyl methane sulfonate, cds1Delta mutants display a complete checkpoint defect. We have identified proteins downstream of Cds1 required for checkpoint-dependant slowing, including the structure-specific endonuclease Mus81 and the helicase Rqh1, which are implicated in replication fork stability and the negative regulation of recombination. Removing Rhp51, the Rad51 recombinase homologue, suppresses the slowing defect of rqh1Delta mutants, but not that of mus81Delta mutant, defining an epistatic pathway in which mus81 is epistatic to rhp51 and rhp51 is epistatic to rqh1. We propose that restraining recombination is required for the slowing of replication in response to DNA damage.
摘要
S期DNA损伤检查点会在复制过程中响应损伤而减缓DNA合成速率。在裂殖酵母粟酒裂殖酵母中,Cds1作为S期特异性检查点效应激酶,是检查点信号传导和复制减缓所必需的;在用烷化剂甲磺酸甲酯处理后,cds1Δ突变体表现出完全的检查点缺陷。我们已经鉴定出Cds1下游的蛋白质,这些蛋白质是检查点依赖性减缓所必需的,包括结构特异性核酸内切酶Mus81和解旋酶Rqh1,它们与复制叉稳定性和重组的负调控有关。去除Rad51重组酶同源物Rhp51可抑制rqh1Δ突变体的减缓缺陷,但不能抑制mus81Δ突变体的减缓缺陷,从而确定了一种上位性途径,其中mus81对rhp51上位,rhp51对rqh1上位。我们提出,抑制重组是响应DNA损伤而减缓复制所必需的。
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