Tsunaka Yasuo, Ohtomo Hideaki, Morikawa Kosuke, Nishimura Yoshifumi
Graduate School of Medical Life Science, Yokohama City University, 1-7-29 Suehiro-cho, Tsurumi-ku, Yokohama 230-0045, Japan.
Department of Gene Mechanisms, Graduate School of Biostudies, Kyoto University, Yoshida-konoemachi, Sakyo-ku, Kyoto 606-8501, Japan.
iScience. 2020 Oct 6;23(10):101641. doi: 10.1016/j.isci.2020.101641. eCollection 2020 Oct 23.
The FACT (facilitates chromatin transcription) complex, comprising SPT16 and SSRP1, conducts structural alterations during nucleosome unwrapping. Our previous cryoelectron microscopic (cryo-EM) analysis revealed the first intermediate structure of an unwrapped nucleosome with human FACT, in which 112-bp DNA and the phosphorylated intrinsically disordered (pAID) segment of SPT16 jointly wrapped around the histone core instead of 145-bp DNA. Using NMR, here we clarified that the histone H3 N-terminal tails, unobserved in the cryo-EM structure, adopt two different conformations reflecting their asymmetric locations at entry/exit sites: one corresponds to the original nucleosome site buried in two DNA gyres (DNA side), whereas the other, comprising pAID and DNA, is more exposed to the solvent (pAID side). NMR real-time monitoring showed that H3 acetylation is faster on the pAID side than on the DNA side. Our findings highlight that accessible conformations of H3 tails are created by the replacement of nucleosomal DNA with pAID.
由SPT16和SSRP1组成的FACT(促进染色质转录)复合物在核小体解旋过程中进行结构改变。我们之前的冷冻电子显微镜(cryo-EM)分析揭示了与人类FACT结合的解旋核小体的首个中间结构,其中112-bp DNA和SPT16的磷酸化内在无序(pAID)片段共同缠绕在组蛋白核心周围,而非145-bp DNA。在此,我们利用核磁共振(NMR)明确了在冷冻电子显微镜结构中未观察到的组蛋白H3 N端尾巴呈现出两种不同构象,这反映了它们在进出位点的不对称位置:一种对应于埋在两个DNA螺旋中的原始核小体位点(DNA侧),而另一种包含pAID和DNA,更暴露于溶剂中(pAID侧)。NMR实时监测表明,H3在pAID侧的乙酰化比在DNA侧更快。我们的研究结果突出表明,H3尾巴的可及构象是通过用pAID取代核小体DNA而产生的。
Zotero 插件
