首页> 美国卫生研究院文献>PLoS Genetics >Connecting Replication and Repair: YoaA a Helicase-Related Protein Promotes Azidothymidine Tolerance through Association with Chi an Accessory Clamp Loader Protein
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Connecting Replication and Repair: YoaA a Helicase-Related Protein Promotes Azidothymidine Tolerance through Association with Chi an Accessory Clamp Loader Protein

机译:连接复制和修复:与解旋酶相关的蛋白质YoaA通过与辅助夹具装载蛋白Chi的缔合促进对叠氮胸苷的耐受性

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摘要

Elongating DNA polymerases frequently encounter lesions or structures that impede progress and require repair before DNA replication can be completed. Therefore, directing repair factors to a blocked fork, without interfering with normal replication, is important for proper cell function, and it is a process that is not well understood. To study this process, we have employed the chain-terminating nucleoside analog, 3’ azidothymidine (AZT) and the E. coli genetic system, for which replication and repair factors have been well-defined. By using high-expression suppressor screens, we identified yoaA, encoding a putative helicase, and holC, encoding the Chi component of the replication clamp loader, as genes that promoted tolerance to AZT. YoaA is a putative Fe-S helicase in the XPD/RAD3 family for which orthologs can be found in most bacterial genomes; E. coli has a paralog to YoaA, DinG, which possesses 5’ to 3’ helicase activity and an Fe-S cluster essential to its activity. Mutants in yoaA are sensitive to AZT exposure; dinG mutations cause mild sensitivity to AZT and exacerbate the sensitivity of yoaA mutant strains. Suppression of AZT sensitivity by holC or yoaA was mutually codependent and we provide evidence here that YoaA and Chi physically interact. Interactions of Chi with single-strand DNA binding protein (SSB) and with Psi were required to aid AZT tolerance, as was the proofreading 3’ exonuclease, DnaQ. Our studies suggest that repair is coupled to blocked replication through these interactions. We hypothesize that SSB, through Chi, recruits the YoaA helicase to replication gaps and that unwinding of the nascent strand promotes repair and AZT excision. This recruitment prevents the toxicity of helicase activity and aids the handoff of repair with replication factors, ensuring timely repair and resumption of replication.
机译:延长的DNA聚合酶经常遇到损害进展的损伤或结构,需要修复才能完成DNA复制。因此,在不影响正常复制的情况下将修复因子引导至受阻的叉子对于细胞的正常功能很重要,而且这一过程尚未得到很好的理解。为了研究这一过程,我们采用了链终止核苷类似物3'叠氮胸苷(AZT)和大肠杆菌的遗传系统,其复制和修复因子已得到明确定义。通过使用高表达抑制子筛选,我们鉴定了编码推定解旋酶的yoaA和编码复制钳装载器的Chi成分的holC,作为促进对AZT的耐受性的基因。 YoaA是XPD / RAD3家族中推定的Fe-S解旋酶,在大多数细菌基因组中都可以找到直系同源物。大肠杆菌与YoaA的同源物DinG,具有5'到3'的解旋酶活性,以及​​对其活性至关重要的Fe-S簇。 yoaA中的突变体对AZT暴露敏感; dinG突变引起对AZT的中等敏感性,并加剧了yoaA突变株的敏感性。 holC或yoaA对AZT敏感性的抑制作用是相互依存的,我们在此提供了YoaA和Chi物理相互作用的证据。需要Chi与单链DNA结合蛋白(SSB)和Psi的相互作用来增强AZT耐受性,而校对3'核酸外切酶DnaQ也是如此。我们的研究表明,修复通过这些相互作用与复制受阻有关。我们假设SSB通过Chi募集YoaA解旋酶以复制缺口,而新生链的解链促进修复和AZT切除。这种募集可防止解旋酶活性的毒性,并有助于复制因子的修复,确保及时修复和恢复复制。

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