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γH2A 与 Brc1 结合以维持 S 期基因组完整性。

gammaH2A binds Brc1 to maintain genome integrity during S-phase.

机构信息

Department of Molecular Biology, The Scripps Research Institute, La Jolla, CA, USA.

出版信息

EMBO J. 2010 Mar 17;29(6):1136-48. doi: 10.1038/emboj.2009.413. Epub 2010 Jan 21.

Abstract

ATM(Tel1) and ATR(Rad3) checkpoint kinases phosphorylate the C-terminus of histone H2AX (H2A in yeasts) in chromatin flanking DNA damage, establishing a recruitment platform for checkpoint and repair proteins. Phospho-H2A/X (gammaH2A/X)-binding proteins at double-strand breaks (DSBs) have been characterized, but those required for replication stress responses are unknown. Here, we present genetic, biochemical, small angle X-ray scattering (SAXS), and X-ray structural studies of the Schizosaccharomyces pombe Brc1, a 6-BRCT-domain protein that is structurally related to Saccharomyces cerevisiae Rtt107 and mammalian PTIP. Brc1 binds gammaH2A to form spontaneous and DNA damage-induced nuclear foci. Spontaneous Brc1 foci colocalize with ribosomal DNA repeats, a region prone to fork pausing and genomic instability, whereas DNA damage-induced Brc1 foci colocalize with DSB response factors. gammaH2A binding is critical for Brc1 function. The 1.45 A resolution crystal structure of Brc1-gammaH2A complex shows how variable BRCT insertion loops sculpt tandem-BRCT phosphoprotein-binding pockets to facilitate unique phosphoprotein-interaction specificities, and unveils an acidic DNA-mimicking Brc1 surface. From these results, Brc1 docking to gammaH2A emerges as a critical chromatin-specific response to replication-associated DNA damage.

摘要

ATM(Tel1)和 ATR(Rad3)检查点激酶在 DNA 损伤侧翼的染色质中磷酸化组蛋白 H2AX(酵母中的 H2A)的 C 末端,为检查点和修复蛋白建立募集平台。已经对双链断裂(DSBs)处的磷酸化 H2A/X(γH2A/X)结合蛋白进行了表征,但对于复制应激反应所需的蛋白仍不清楚。在这里,我们介绍了裂殖酵母 Brc1 的遗传、生化、小角度 X 射线散射(SAXS)和 X 射线结构研究,Brc1 是一种具有 6-BRCT 结构域的蛋白质,在结构上与酿酒酵母 Rtt107 和哺乳动物 PTIP 相关。Brc1 与 γH2A 结合形成自发和 DNA 损伤诱导的核焦点。自发的 Brc1 焦点与核糖体 DNA 重复序列共定位,这是一个容易发生叉暂停和基因组不稳定性的区域,而 DNA 损伤诱导的 Brc1 焦点与 DSB 反应因子共定位。γH2A 结合对于 Brc1 的功能至关重要。Brc1-γH2A 复合物的 1.45Å分辨率晶体结构显示了可变 BRCT 插入环如何塑造串联 BRCT 磷酸化蛋白结合口袋,以促进独特的磷酸化蛋白相互作用特异性,并揭示了一个酸性的 DNA 模拟 Brc1 表面。从这些结果中可以看出,Brc1 与 γH2A 的对接是对与复制相关的 DNA 损伤的一种关键的染色质特异性反应。

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