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使用甲基-TROSY NMR 研究去稳定核小体的动力学。

Investigating the Dynamics of Destabilized Nucleosomes Using Methyl-TROSY NMR.

机构信息

Departments of Chemistry, Molecular Genetics, and Biochemistry , University of Toronto , Toronto , Ontario M5S 1A8 , Canada.

Department of Chemistry and Biochemistry , University of Colorado , Boulder , Colorado 80309 , United States.

出版信息

J Am Chem Soc. 2018 Apr 11;140(14):4774-4777. doi: 10.1021/jacs.8b00931. Epub 2018 Mar 28.

Abstract

The nucleosome core particle (NCP), comprised of histone proteins wrapped with ∼146 base pairs of DNA, provides both protection and controlled access to DNA so as to regulate vital cellular processes. High-resolution structures of nucleosomes and nucleosome complexes have afforded a clear understanding of the structural role of NCPs, but a detailed description of the dynamical properties that facilitate DNA-templated processes is only beginning to emerge. Using methyl-TROSY NMR approaches we evaluate the effect of point mutations designed to perturb key histone interfaces that become destabilized during nucleosome remodeling in an effort to probe NCP plasticity. Notably the NCP retains its overall structural integrity, yet relaxation experiments of mutant nucleosomes reveal significant dynamics within a central histone interface associated with alternative NCP conformations populated to as much as 15% under low salt conditions. This work highlights the inherent plasticity of NCPs and establishes methyl-TROSY NMR as a valuable compliment to current single molecule methods in quantifying NCP dynamic properties.

摘要

核小体核心颗粒(NCP)由包裹着约 146 个碱基对 DNA 的组蛋白组成,为 DNA 提供保护和控制访问,从而调节重要的细胞过程。核小体和核小体复合物的高分辨率结构使人们清楚地了解了 NCP 的结构作用,但对于促进 DNA 模板过程的动态特性的详细描述才刚刚开始出现。我们使用甲基-TROSY NMR 方法评估了设计用于扰乱关键组蛋白界面的点突变的影响,这些界面在核小体重塑过程中变得不稳定,以探测 NCP 的可塑性。值得注意的是,NCP 保持其整体结构完整性,但突变核小体的弛豫实验揭示了与替代 NCP 构象相关的中心组蛋白界面内的显著动力学,在低盐条件下,这些构象的丰度可达 15%。这项工作强调了 NCP 的固有可塑性,并确立了甲基-TROSY NMR 作为当前单分子方法在定量 NCP 动态特性方面的有力补充。

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