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YL1,SRCAP 染色质重塑亚基识别 H2A.Z 的结构基础。

Structural basis of H2A.Z recognition by SRCAP chromatin-remodeling subunit YL1.

机构信息

National Laboratory of Biomacromolecules, Institute of Biophysics, Chinese Academy of Sciences, Beijing, China.

University of Chinese Academy of Sciences, Beijing, China.

出版信息

Nat Struct Mol Biol. 2016 Apr;23(4):317-23. doi: 10.1038/nsmb.3190. Epub 2016 Mar 14.

Abstract

Histone variant H2A.Z, a universal mark of dynamic nucleosomes flanking gene promoters and enhancers, is incorporated into chromatin by SRCAP (SWR1), an ATP-dependent, multicomponent chromatin-remodeling complex. The YL1 (Swc2) subunit of SRCAP (SWR1) plays an essential role in H2A.Z recognition, but how it achieves this has been unclear. Here, we report the crystal structure of the H2A.Z-binding domain of Drosophila melanogaster YL1 (dYL1-Z) in complex with an H2A.Z-H2B dimer at 1.9-Å resolution. The dYL1-Z domain adopts a new whip-like structure that wraps over H2A.Z-H2B, and preferential recognition is largely conferred by three residues in loop 2, the hyperacidic patch and the extended αC helix of H2A.Z. Importantly, this domain is essential for deposition of budding yeast H2A.Z in vivo and SRCAP (SWR1)-catalyzed histone H2A.Z replacement in vitro. Our studies distinguish YL1-Z from known H2A.Z chaperones and suggest a hierarchical mechanism based on increasing binding affinity facilitating H2A.Z transfer from SRCAP (SWR1) to the nucleosome.

摘要

组蛋白变体 H2A.Z 是一种普遍存在的标记,存在于基因启动子和增强子侧翼的动态核小体中,由 SRCAP(SWR1)将其掺入染色质中,SRCAP(SWR1)是一种依赖 ATP 的多成分染色质重塑复合物。SRCAP(SWR1)中的 YL1(Swc2)亚基在 H2A.Z 的识别中起着至关重要的作用,但它是如何实现这一目标的还不清楚。在这里,我们报告了黑腹果蝇 YL1(dYL1-Z)的 H2A.Z 结合域与 H2A.Z-H2B 二聚体复合物的晶体结构,分辨率为 1.9-Å。dYL1-Z 结构域采用了一种新的鞭状结构,缠绕在 H2A.Z-H2B 上,主要通过 H2A.Z 上的环 2、超酸性补丁和延伸的αC 螺旋中的三个残基进行优先识别。重要的是,该结构域对于体内芽殖酵母 H2A.Z 的沉积和体外 SRCAP(SWR1)催化的组蛋白 H2A.Z 取代都是必需的。我们的研究将 YL1-Z 与已知的 H2A.Z 伴侣蛋白区分开来,并提出了一种基于增加结合亲和力的分层机制,促进 H2A.Z 从 SRCAP(SWR1)转移到核小体。

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