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细菌视紫红质在古紫质-2三聚体结构中的结构作用。

Structural role of bacterioruberin in the trimeric structure of archaerhodopsin-2.

作者信息

Yoshimura Keiko, Kouyama Tsutomu

机构信息

Department of Physics, Graduate School of Science, Nagoya University, Chikusa-ku, Nagoya 464-8602, Japan.

出版信息

J Mol Biol. 2008 Feb 1;375(5):1267-81. doi: 10.1016/j.jmb.2007.11.039. Epub 2007 Nov 22.

DOI:10.1016/j.jmb.2007.11.039
PMID:18082767
Abstract

Archaerhodopsin-2 (aR2), a retinal protein-carotenoid complex found in the claret membrane of Halorubrum sp. aus-2, functions as a light-driven proton pump. In this study, the membrane fusion method was utilized to prepare trigonal P321 crystals (a=b=98.2 A, c=56.2 A) and hexagonal P6(3) crystals (a=b=108.8 A, c=220.7 A). The trigonal crystal is made up of stacked membranes in which the aR2 trimers are arranged on a honeycomb lattice. Similar membranous structures are found in the hexagonal crystal, but four membrane layers with different orientations are contained in the unit cell. In these crystals, the carotenoid bacterioruberin [5,32-bis(2-hydroxypropan-2-yl)-2,8,12,16,21,25,29,35-octamethylhexatriaconta-6,8,10,12,14,16,18,20,22,24,26,28,30-tridecaene-2,35-diol] binds to crevices between the subunits of the trimer. Its polyene chain is inclined from the membrane normal by an angle of about 20 degrees and, on the cytoplasmic side, it is surrounded by helices AB and DE of neighbouring subunits. This peculiar binding mode suggests that bacterioruberin plays a striking structural role for the trimerization of aR2. When compared with the aR2 structure in another crystal form containing no bacterioruberin, the proton release channel takes a more closed conformation in the P321 or P6(3) crystal; i.e., the native conformation of protein is stabilized in the trimeric protein-bacterioruberin complex. Interestingly, most residues participating in the trimerization are not conserved in bacteriorhodopsin, a homologous protein capable of forming a trimeric structure in the absence of bacterioruberin. Despite a large alteration in the amino acid sequence, the shape of the intratrimer hydrophobic space filled by lipids is highly conserved between aR2 and bacteriorhodopsin. Since a transmembrane helix facing this space undergoes a large conformational change during the proton pumping cycle, it is feasible that trimerization is an important strategy to capture special lipid components that are relevant to the protein activity.

摘要

古紫质-2(aR2)是一种存在于嗜盐碱红菌aus-2菌膜中的视网膜蛋白-类胡萝卜素复合物,具有光驱动质子泵的功能。在本研究中,采用膜融合方法制备了三方晶系P321晶体(a = b = 98.2 Å,c = 56.2 Å)和六方晶系P6(3)晶体(a = b = 108.8 Å,c = 220.7 Å)。三方晶体由堆叠的膜组成,其中aR2三聚体排列在蜂窝晶格上。在六方晶体中发现了类似的膜结构,但晶胞中包含四个不同取向的膜层。在这些晶体中,类胡萝卜素细菌红素[5,32-双(2-羟丙基)-2,8,12,16,21,25,29,35-八甲基三十六碳-6,8,10,12,14,16,18,20,22,24,26,28,30-十三碳烯-2,35-二醇]与三聚体亚基之间的缝隙结合。其多烯链与膜法线倾斜约20度角,在细胞质一侧,它被相邻亚基的AB和DE螺旋包围。这种特殊的结合模式表明细菌红素在aR2三聚化过程中发挥了显著的结构作用。与另一种不含细菌红素的晶体形式中的aR2结构相比,质子释放通道在P321或P6(3)晶体中处于更封闭的构象;即蛋白质的天然构象在三聚体蛋白质-细菌红素复合物中得到稳定。有趣的是,参与三聚化的大多数残基在细菌视紫红质中并不保守,细菌视紫红质是一种在没有细菌红素的情况下能够形成三聚体结构的同源蛋白。尽管氨基酸序列有很大变化,但aR2和细菌视紫红质之间由脂质填充的三聚体内疏水空间的形状高度保守。由于面向该空间的跨膜螺旋在质子泵循环过程中会发生很大的构象变化,因此三聚化是捕获与蛋白质活性相关的特殊脂质成分的重要策略是可行的。

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