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首页> 外文期刊>Journal of Molecular Biology >The Biophysical Basis for Phosphorylation-Enhanced DNA-Binding Autoinhibition of the ETS1 Transcription Factor
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The Biophysical Basis for Phosphorylation-Enhanced DNA-Binding Autoinhibition of the ETS1 Transcription Factor

机译:磷酸化增强DNA结合的生物物理基础自体抑制ETS1转录因子

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摘要

The eukaryotic transcription factor ETS1 is regulated by an intrinsically disordered serine-rich region (SRR) that transiently associates with the adjacent ETS domain to inhibit DNA binding. In this study, we further elucidated the physicochemical basis for ETS1 autoinhibition by characterizing the interaction of its ETS domain with a series of synthetic peptides corresponding to the SRR. Binding is driven by the hydrophobic effect and enhanced electrostatically by phosphorylation of serines adjacent to aromatic residues in the amphipathic SRR. Structural characterization of the dynamic peptide/protein complex by NMR spectroscopy and X-ray crystallography revealed multiple modes of binding that lead to autoinhibition by synergistically blocking the DNA-binding interface of the ETS domain and stabilizing an appended helical inhibitory module against allosterically induced unfolding. Consistent with these conclusions, the SRR peptide does not interact with DNA-bound ETS1. In addition, we found that the ETS1 SRR phosphopeptide binds to distantly related PU.1 in vitro, indicating that autoinhibition exploits features of the ETS domain that are conserved across this family of transcription factors. (C) 2018 Elsevier Ltd. All rights reserved.
机译:真核转录因子ETS1由本质上无序的富含丝氨酸的富集区域(SRR)调节,其瞬时与相邻的ETS结构域缔合以抑制DNA结合。在这项研究中,我们进一步阐明了ETS1自动抑制的物理化学基础,通过表征其ETS结构域与对应于SRR的一系列合成肽的相互作用。结合由疏水效果驱动并通过邻近芳族残基的丝氨酸磷酸化静电增强。通过NMR光谱和X射线晶体术的动态肽/蛋白质复合物的结构表征显示了通过协同阻断ETS结构域的DNA结合界面和稳定Appended Helical抑制模块,通过协同阻断Astensed Helical抑制模块而导致自动抑制的多种结合模式。与这些结论一致,SRR肽不与DNA结合的ETS1相互作用。此外,我们发现ETS1 SRR磷酸肽在体外结合远处相关的PU.1,表明自动抑制挖掘在该系列转录因子中保存的ETS结构域的特征。 (c)2018年elestvier有限公司保留所有权利。

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