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DNA ligase III acts as a DNA strand break sensor in the cellular orchestration of DNA strand break repair

机译:DNA连接酶III在DNA链断裂修复的细胞编排中充当DNA链断裂传感器

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摘要

In the current model of DNA SSBR, PARP1 is regarded as the sensor of single-strand breaks (SSBs). However, biochemical studies have implicated LIG3 as another possible SSB sensor. Using a laser micro-irradiation protocol that predominantly generates SSBs, we were able to demonstrate that PARP1 is dispensable for the accumulation of different single-strand break repair (SSBR) proteins at sites of DNA damage in live cells. Furthermore, we show in live cells for the first time that LIG3 plays a role in mediating the accumulation of the SSBR proteins XRCC1 and PNKP at sites of DNA damage. Importantly, the accumulation of LIG3 at sites of DNA damage did not require the BRCT domain-mediated interaction with XRCC1. We were able to show that the N-terminal ZnF domain of LIG3 plays a key role in the enzyme's SSB sensing function. Finally, we provide cellular evidence that LIG3 and not PARP1 acts as the sensor for DNA damage caused by the topoisomerase I inhibitor, irinotecan. Our results support the existence of a second damage-sensing mechanism in SSBR involving the detection of nicks in the genome by LIG3.
机译:在当前的DNA SSBR模型中,PARP1被视为单链断裂(SSB)的传感器。但是,生化研究表明LIG3是另一种可能的SSB传感器。使用主要产生SSB的激光微辐射方案,我们能够证明PARP1对于活细胞DNA损伤部位不同单链断裂修复(SSBR)蛋白的积累是可有可无的。此外,我们首次在活细胞中显示LIG3在介导SSBR蛋白XRCC1和PNKP在DNA损伤部位的积累中起着作用。重要的是,LIG3在DNA损伤位点的积累不需要BRCT域介导的与XRCC1的相互作用。我们能够证明,LIG3的N端ZnF结构域在酶的SSB感应功能中起关键作用。最后,我们提供了细胞证据,表明LIG3而非PARP1充当拓扑异构酶I抑制剂伊立替康引起的DNA损伤的传感器。我们的结果支持SSBR中存在第二种损伤感应机制,涉及通过LIG3检测基因组中的缺口。

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