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冷冻电镜结构Native 视紫红质二聚体在纳米盘。

Cryo-EM structure of the native rhodopsin dimer in nanodiscs.

机构信息

Department of Biochemistry, University of Toronto, Toronto, Ontario M5S 1A8, Canada.

Department of Molecular Structural Biology, Max-Planck Institute of Biochemistry, 82152 Martinsried, Germany.

出版信息

J Biol Chem. 2019 Sep 27;294(39):14215-14230. doi: 10.1074/jbc.RA119.010089. Epub 2019 Aug 9.

Abstract

Imaging of rod photoreceptor outer-segment disc membranes by atomic force microscopy and cryo-electron tomography has revealed that the visual pigment rhodopsin, a prototypical class A G protein-coupled receptor (GPCR), can organize as rows of dimers. GPCR dimerization and oligomerization offer possibilities for allosteric regulation of GPCR activity, but the detailed structures and mechanism remain elusive. In this investigation, we made use of the high rhodopsin density in the native disc membranes and of a bifunctional cross-linker that preserves the native rhodopsin arrangement by covalently tethering rhodopsins via Lys residue side chains. We purified cross-linked rhodopsin dimers and reconstituted them into nanodiscs for cryo-EM analysis. We present cryo-EM structures of the cross-linked rhodopsin dimer as well as a rhodopsin dimer reconstituted into nanodiscs from purified monomers. We demonstrate the presence of a preferential 2-fold symmetrical dimerization interface mediated by transmembrane helix 1 and the cytoplasmic helix 8 of rhodopsin. We confirmed this dimer interface by double electron-electron resonance measurements of spin-labeled rhodopsin. We propose that this interface and the arrangement of two protomers is a prerequisite for the formation of the observed rows of dimers. We anticipate that the approach outlined here could be extended to other GPCRs or membrane receptors to better understand specific receptor dimerization mechanisms.

摘要

利用原子力显微镜和冷冻电镜断层扫描对杆状光感受器外段盘膜的成像研究表明,视紫红质(一种典型的 A 类 G 蛋白偶联受体(GPCR))可以排列成二聚体列。GPCR 二聚化和寡聚化为 GPCR 活性的变构调节提供了可能性,但详细的结构和机制仍然难以捉摸。在这项研究中,我们利用了天然盘膜中高浓度的视紫红质和一种双功能交联剂,该交联剂通过赖氨酸残基侧链共价键将视紫红质连接起来,从而保持天然视紫红质的排列。我们纯化了交联的视紫红质二聚体,并将其重新组装成纳米盘进行冷冻电镜分析。我们提出了交联的视紫红质二聚体的冷冻电镜结构,以及从纯化的单体中重新组装成纳米盘的视紫红质二聚体的结构。我们证明了存在一个由跨膜螺旋 1 和视紫红质胞质螺旋 8 介导的优先 2 倍对称二聚化界面。我们通过对自旋标记视紫红质的双电子-电子共振测量证实了这个二聚体界面。我们提出,这个界面和两个前体的排列是形成观察到的二聚体列的先决条件。我们预计,这里概述的方法可以扩展到其他 GPCR 或膜受体,以更好地理解特定的受体二聚化机制。

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