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首页> 外文期刊>Molecular biology reports >A homologue of the Rad18 postreplication repair gene is required for DNA damage responses throughout the fission yeast cell cycle.
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A homologue of the Rad18 postreplication repair gene is required for DNA damage responses throughout the fission yeast cell cycle.

机译:Rad18复制后修复基因的同源物是整个裂殖酵母细胞周期内DNA损伤反应所必需的。

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摘要

Cells activate DNA repair pathways and cell cycle checkpoints when they suffer damage to their genome. They also activate tolerance pathways that facilitate survival. In Escherichia coli, a mechanism known as postreplication repair (PRR) is used to bypass lesions that would otherwise present a physical block to DNA polymerase. PRR has also been proposed to occur in eukaryotic cells, although the partitioning of DNA synthesis to a discrete S-phase would suggest that it is only operative within a defined period of the cell cycle. Eukaryotic PRR has been most extensively studied in the budding yeast Saccharomyces cerevisiae. Two important genes for components of this repair pathway are RAD6, which encodes an ubiquitin-conjugating enzyme, and RAD18, which encodes a RING-finger protein and forms a heterodimer with Rad6p. Rad18p can also bind to DNA. We report here the identification of the Schizosaccharomyces pombe homologue of RAD18, which we have denoted rhp18. rhp18 mutants are hypersensitive to DNA-damaging agents, but show this hypersensitivity throughout the cell cycle. rhp18 mutants are characterised by a longer than usual DNA damage checkpoint arrest that is required for their residual viability following irradiation. Genetic analyses show that rhp18 controls a unique DNA damage repair/tolerance pathway that extends beyond the requirement to tolerate damage during S-phase, suggesting a broader definition of the function of this eukaryotic PRR protein.
机译:当细胞遭受基因组破坏时,它们会激活DNA修复途径和细胞周期检查点。它们还激活促进生存的耐受途径。在大肠杆菌中,一种称为复制后修复(PRR)的机制可用于绕过病变,否则这些病变将对DNA聚合酶产生物理阻碍。还提出了PRR在真核细胞中发生,尽管将DNA合成划分为离散的S期将表明它仅在细胞周期的限定时间内起作用。真核PRR已在发芽酵母酿酒酵母中得到了最广泛的研究。该修复途径的两个重要基因是RAD6(其编码泛素结合酶)和RAD18(其编码RING手指蛋白并与Rad6p形成异二聚体)。 Rad18p也可以与DNA结合。我们在这里报告了RAD18的粟酒裂殖酵母同源物的鉴定,我们将其标记为rhp18。 rhp18突变体对DNA破坏剂非常敏感,但在整个细胞周期中都表现出这种超敏性。 rhp18突变体的特点是,比正常的DNA损伤检查点停滞时间更长,这是辐射后其剩余生存能力所必需的。遗传分析表明,rhp18控制独特的DNA损伤修复/耐受途径,该途径超出了在S期耐受耐受的要求,这表明该真核PRR蛋白功能的定义更为广泛。

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