Structure of bovine rhodopsin in a trigonal crystal form

被引:636
|
作者
Li, J
Edwards, PC
Burghammer, M
Villa, C
Schertler, GFX
机构
[1] MRC, Mol Biol Lab, Cambridge CB2 2QH, England
[2] European Synchrotron Radiat Facil, F-38043 Grenoble, France
关键词
G protein-coupled receptor; G protein activation; ligand binding pocket; membrane protein structure; visual pigments;
D O I
10.1016/j.jmb.2004.08.090
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
We have determined the structure of bovine rhodopsin at 2.65 Angstrom resolution using untwinned native crystals in the space group P3(1), by molecular replacement from the 2.8 Angstrom model (1F88) solved in space group P4(1). The new structure reveals mechanistically important details unresolved previously, which are considered in the membrane context by docking the structure into a cryo-electron microscopy map of 2D crystals. Kinks in the transmembrane helices facilitate inter-helical polar interactions. Ordered water molecules extend the hydrogen bonding networks, linking Trp265 in the retinal binding pocket to the NPxxY motif near the cytoplasmic boundary, and the Glu113 counterion for the protonated Schiff base to the extracellular surface. Glu113 forms a complex with a water molecule hydrogen bonded between its main chain and side-chain oxygen atoms. This can be expected to stabilise the salt-bridge with the protonated Schiff base linking the 11-cis-retinal to Lys296. The cytoplasmic ends of helices H5 and H6 have been extended by one turn. The G-protein interaction sites mapped to the cytoplasmic ends of H5 and H6 and a spiral extension of H5 are elevated above the bilayer. There is a surface cavity next to the conserved Glu134-Arg135 ion pair. The cytoplasmic loops have the highest temperature factors in the structure, indicative of their flexibility when not interacting with G protein or regulatory proteins. An ordered detergent molecule is seen wrapped around the kink in H6, stabilising the structure around the potential hinge in H6. These findings provide further explanation for the stability of the dark state structure. They support a mechanism for the activation, initiated by photo-isomerisation of the chromophore to its all-trans form, that involves pivoting movements of kinked helices, which, while maintaining hydrophobic contacts in the membrane interior, can be coupled to amplified translation of the helix ends near the membrane surfaces. (C) 2004 Elsevier Ltd. All rights reserved.
引用
收藏
页码:1409 / 1438
页数:30
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