首页> 外文期刊>Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses >Local regulation of the Srs2 helicase by the SUMO-like domain protein Esc2 promotes recombination at sites of stalled replication
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Local regulation of the Srs2 helicase by the SUMO-like domain protein Esc2 promotes recombination at sites of stalled replication

机译:SUMO样结构域蛋白Esc2对Srs2解旋酶的局部调节促进了停滞复制位点的重组

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摘要

Accurate completion of replication relies on the ability of cells to activate error-free recombination-mediated DNA damage bypass at sites of perturbed replication. However, as anti-recombinase activities are also recruited to replication forks, how recombination-mediated damage bypass is enabled at replication stress sites remained puzzling. Here we uncovered that the conserved SUMO-like domain-containing Saccharomyces cerevisiae protein Esc2 facilitates recombination-mediated DNA damage tolerance by allowing optimal recruitment of the Rad51 recombinase specifically at sites of perturbed replication. Mechanistically, Esc2 binds stalled replication forks and counteracts the anti-recombinase Srs2 helicase via a two-faceted mechanism involving chromatin recruitment and turnover of Srs2. Importantly, point mutations in the SUMO-like domains of Esc2 that reduce its interaction with Srs2 cause suboptimal levels of Rad51 recruitment at damaged replication forks. In conclusion, our results reveal how recombination-mediated DNA damage tolerance is locally enabled at sites of replication stress and globally prevented at undamaged replicating chromosomes.
机译:复制的准确完成取决于细胞在干扰复制位点激活无错重组介导的DNA损伤旁路的能力。但是,由于抗重组酶活性也被募集到复制叉中,因此如何在复制应激位点启用重组介导的损伤旁路仍然令人费解。在这里,我们发现保守的含SUMO样结构域的酿酒酵母蛋白Esc2通过允许Rad51重组酶特异性地在扰动复制位点进行最佳募集,促进重组介导的DNA损伤耐受性。从机理上讲,Esc2结合停滞的复制叉,并通过涉及染色质募集和Srs2周转的两方面机制来抵消抗重组酶Srs2解旋酶。重要的是,Esc2的SUMO样结构域中的点突变会减少其与Srs2的相互作用,从而导致损坏的复制叉处Rad51募集的次优水平。总之,我们的研究结果揭示了重组介导的DNA损伤耐受性是如何在复制压力位点局部启用的,而在未损坏的复制染色体上是全面阻止的。

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