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The deSUMOylase SENP2 coordinates homologous recombination and nonhomologous end joining by independent mechanisms

机译:deSUMOylase SENP2通过独立的机制协调同源重组和非同源末端连接

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摘要

SUMOylation (small ubiquitin-like modifier) in the DNA double-strand break (DSB) response regulates recruitment, activity, and clearance of repair factors. However, our understanding of a role for deSUMOylation in this process is limited. Here we identify different mechanistic roles for deSUMOylation in homologous recombination (HR) and nonhomologous end joining (NHEJ) through the investigation of the deSUMOylase SENP2. We found that regulated deSUMOylation of MDC1 prevents excessive SUMOylation and its RNF4-VCP mediated clearance from DSBs, thereby promoting NHEJ. In contrast, we show that HR is differentially sensitive to SUMO availability and SENP2 activity is needed to provide SUMO. SENP2 is amplified as part of the chromosome 3q amplification in many cancers. Increased SENP2 expression prolongs MDC1 focus retention and increases NHEJ and radioresistance. Collectively, our data reveal that deSUMOylation differentially primes cells for responding to DSBs and demonstrates the ability of SENP2 to tune DSB repair responses.
机译:DNA双链断裂(DSB)反应中的SUMOylation(小的泛素样修饰剂)调节募集,活性和修复因子的清除。但是,我们对脱SUMOylation在此过程中的作用的理解是有限的。在这里,我们通过对deSUMOylase SENP2的研究,确定了在同源重组(HR)和非同源末端连接(NHEJ)中deSUMOylation的不同机制作用。我们发现,受调节的MDC1的deSUMOylation可防止过度的SUMOylation及其RNF4-VCP介导的DSB清除,从而促进NHEJ。相比之下,我们显示HR对SUMO可用性具有不同的敏感性,并且需要SENP2活性才能提供SUMO。在许多癌症中,SENP2被扩增为染色体3q扩增的一部分。 SENP2表达的增加延长了MDC1的焦点保持力,并增加了NHEJ和抗辐射性。总的来说,我们的数据揭示了deSUMOylation差异地引发了细胞对DSB的反应,并证明了SENP2调节DSB修复反应的能力。

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