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泛素化的 9-1-1 检查点钳独立的 rad6-rad18 和 DNA 损伤。

Ubiquitylation of the 9-1-1 checkpoint clamp is independent of rad6-rad18 and DNA damage.

机构信息

Cancer Research UK London Research Institute, Clare Hall Laboratories, Blanche Lane, South Mimms EN6 3LD, UK.

出版信息

Cell. 2010 Jun 11;141(6):1080-7. doi: 10.1016/j.cell.2010.04.039.

Abstract

A recent report proposed a function of the ubiquitin conjugation factors Rad6 and Rad18 comparable to the bacterial SOS response, controlling damage-induced transcriptional activation and contributing to checkpoint signaling. The relevant ubiquitylation target was identified as budding yeast Rad17, a subunit of the PCNA-like 9-1-1 checkpoint clamp. We report here that in fact all three subunits of the 9-1-1 complex are ubiquitylated. However, in contrast to previous results, we found modification of Rad17 to be independent of DNA damage, the Rad6-Rad18 complex, the putative acceptor site (lysine 197), and loading of the complex onto DNA. Consistently, we were unable to observe enhanced damage sensitivity or defects in checkpoint signaling in a rad17(K197R) mutant. Instead, our findings suggest that ubiquitylation of the 9-1-1 complex may be a background reaction that in some cases can mediate proteasomal degradation.

摘要

最近的一份报告提出了泛素连接因子 Rad6 和 Rad18 的功能类似于细菌 SOS 反应,控制损伤诱导的转录激活,并有助于检查点信号转导。相关的泛素化靶标被鉴定为芽殖酵母 Rad17,PCNA 样 9-1-1 检查点钳的一个亚基。我们在这里报告实际上 9-1-1 复合物的所有三个亚基都被泛素化。然而,与先前的结果相反,我们发现 Rad17 的修饰与 DNA 损伤、Rad6-Rad18 复合物、假定的接受位点(赖氨酸 197)以及复合物在 DNA 上的加载无关。一致地,我们无法观察到 rad17(K197R)突变体中增强的损伤敏感性或检查点信号转导缺陷。相反,我们的研究结果表明,9-1-1 复合物的泛素化可能是一种背景反应,在某些情况下可以介导蛋白酶体降解。

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