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建模兰尼碱受体 N 端结构域连接中央前庭和角夹区。

Modeling a ryanodine receptor N-terminal domain connecting the central vestibule and the corner clamp region.

机构信息

Wadsworth Center, New York State Department of Health, Albany, New York 12201, USA.

出版信息

J Biol Chem. 2013 Jan 11;288(2):903-14. doi: 10.1074/jbc.M112.429670. Epub 2012 Nov 30.

Abstract

Ryanodine receptors (RyRs) form a class of intracellular calcium release channels in various excitable tissues and cells such as muscles and neurons. They are the major cellular mediators of the release of calcium ions from the sarcoplasmic reticulum, an essential step in muscle excitation-contraction coupling. Several crystal structures of skeletal muscle RyR1 peptide fragments have been solved, but these cover less than 15% of the full-length RyR1 sequence. In this study, by combining modeling techniques with sub-nanometer resolution cryo-electron microscopy (cryo-EM) maps, we obtained pseudo-atomic models for RyR fragments consisting of residues 850-1,056 in rabbit RyR1 or residues 861-1,067 in mouse RyR2. These fragments are docked into a domain that connects the central vestibule and corner clamp region of RyR, resulting in a good match of the secondary structure elements in the cryo-EM map and the pseudo-atomic models, which is also consistent with our previous mappings of GFP insertions by cryo-EM and with FRET measurements involving RyR and FK506-binding protein (FKBP). A combined model of the RyR fragment and FKBP docked into the cryo-EM map suggests that the fragment is positioned adjacent to the FKBP-binding site. Its predicted binding interface with FKBP consists primarily of electrostatic contacts and contains several disease-associated mutations. A dynamic interaction between the fragment and an RyR phosphorylation domain, characterized by FRET experiments, also supports the structural predictions of the pseudo-atomic models.

摘要

Ryanodine 受体(RyRs)是各种可兴奋组织和细胞(如肌肉和神经元)中细胞内钙释放通道的一个类别。它们是肌浆网钙离子释放的主要细胞介质,是肌肉兴奋-收缩耦联的关键步骤。已经解决了几种骨骼肌 RyR1 肽片段的晶体结构,但这些结构仅覆盖 RyR1 全长序列的不到 15%。在这项研究中,我们通过将建模技术与亚纳米分辨率冷冻电镜(cryo-EM)图谱相结合,获得了由兔 RyR1 的残基 850-1,056 或鼠 RyR2 的残基 861-1,067 组成的 RyR 片段的拟原子模型。这些片段被对接至连接 RyR 中央前庭和角夹区域的结构域,从而使 cryo-EM 图谱中的二级结构元件与拟原子模型之间具有良好的匹配,这也与我们之前通过 cryo-EM 进行 GFP 插入的映射以及涉及 RyR 和 FK506 结合蛋白(FKBP)的 FRET 测量结果一致。RyR 片段和 FKBP 对接至 cryo-EM 图谱的组合模型表明,该片段位于 FKBP 结合位点附近。其与 FKBP 的预测结合界面主要由静电相互作用组成,并且包含几个与疾病相关的突变。通过 FRET 实验表征的片段与 RyR 磷酸化结构域之间的动态相互作用也支持了拟原子模型的结构预测。

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本文引用的文献

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FEBS J. 2012 Oct;279(20):3952-64. doi: 10.1111/j.1742-4658.2012.08755.x. Epub 2012 Sep 11.
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