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核小体组蛋白 H3 尾部结合配对读取器的可达性。

Accessibility of the histone H3 tail in the nucleosome for binding of paired readers.

机构信息

Department of Pharmacology, University of Colorado School of Medicine, Aurora, CO, 80045, USA.

Department of Biochemistry and Biophysics, University of Rochester Medical Center, Rochester, NY, 14642, USA.

出版信息

Nat Commun. 2017 Nov 14;8(1):1489. doi: 10.1038/s41467-017-01598-x.

Abstract

Combinatorial polyvalent contacts of histone-binding domains or readers commonly mediate localization and activities of chromatin-associated proteins. A pair of readers, the PHD fingers of the protein CHD4, has been shown to bivalently recognize histone H3 tails. Here we describe a mechanism by which these linked but independent readers bind to the intact nucleosome core particle (NCP). Comprehensive NMR, chemical reactivity, molecular dynamics, and fluorescence analyses point to the critical roles of intra-nucleosomal histone-DNA interactions that reduce the accessibility of H3 tails in NCP, the nucleosomal DNA, and the linker between readers in modulating nucleosome- and/or histone-binding activities of the readers. We show that the second PHD finger of CHD4 initiates recruitment to the nucleosome, however both PHDs are required to alter the NCP dynamics. Our findings reveal a distinctive regulatory mechanism for the association of paired readers with the nucleosome that provides an intricate balance between cooperative and individual activities of the readers.

摘要

组蛋白结合域或读取器的组合多价接触通常介导染色质相关蛋白的定位和活性。一对读取器,即蛋白 CHD4 的 PHD 指,已被证明可以二价识别组蛋白 H3 尾部。在这里,我们描述了这些连接但独立的读取器结合完整核小体核心颗粒(NCP)的机制。全面的 NMR、化学反应性、分子动力学和荧光分析指出,核小体内部组蛋白-DNA 相互作用在调节读取器的核小体和/或组蛋白结合活性方面起着关键作用,这些相互作用降低了 NCP 中 H3 尾部、核小体 DNA 和读取器之间连接子的可及性。我们表明,CHD4 的第二个 PHD 指首先募集到核小体,但两个 PHD 都需要改变 NCP 的动力学。我们的发现揭示了配对读取器与核小体结合的独特调节机制,为读取器的协同和单独活性之间提供了精细的平衡。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c709/5686127/d37365a757e2/41467_2017_1598_Fig1_HTML.jpg

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