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细菌视紫红质突变体的振动光谱:发色团异构化扰动色氨酸-86。

Vibrational spectroscopy of bacteriorhodopsin mutants: chromophore isomerization perturbs tryptophan-86.

作者信息

Rothschild K J, Gray D, Mogi T, Marti T, Braiman M S, Stern L J, Khorana H G

机构信息

Physics Department, Boston University, Massachusetts 02215.

出版信息

Biochemistry. 1989 Aug 22;28(17):7052-9. doi: 10.1021/bi00443a041.

DOI:10.1021/bi00443a041
PMID:2819048
Abstract

Fourier transform infrared difference spectra have been obtained for the bR----K and bR----M photoreactions of bacteriorhodopsin mutants with Phe replacements for Trp residues 10, 12, 80, 86, 138, 182, and 189 and Cys replacements for Trp residues 137 and 138. None of the tryptophan mutations caused a significant shift in the retinylidene C = C or C-C stretching frequencies of the visible absorption maximum of the chromophore, it is concluded that none of the tryptophan residues are essential for forming a normal bR570 chromophore. However, a 742-cm-1 negative peak attributed previously to the perturbation of a tryptophan residue during the bR----K photoreaction was found to be absent in the bR----K and bR----M difference spectra of the Trp-86 mutant. On this basis, we conclude that the structure or environment of Trp-86 is altered during the bR----K photoreaction. All of the other Trp----Phe mutants exhibited this band, although its frequency was altered in the Trp-189----Phe mutant. In addition, the Trp-182----Phe mutant exhibited much reduced formation of normal photoproducts relative to the other mutants, as well as peaks indicative of the presence of additional chromophore conformations. A model of bR is discussed in which Trp-86, Trp-182, and Trp-189 form part of a retinal binding pocket. One likely function of these tryptophan groups is to provide the structural constraints needed to prevent chromophore photoisomerization other than at the C13 = C14 double bond.

摘要

已获得细菌视紫红质突变体的傅里叶变换红外差光谱,这些突变体中色氨酸残基10、12、80、86、138、182和189被苯丙氨酸取代,色氨酸残基137和138被半胱氨酸取代,用于细菌视紫红质的bR----K和bR----M光反应。没有一个色氨酸突变导致发色团可见吸收最大值的视黄叉烯C = C或C-C伸缩频率发生显著变化,由此得出结论,没有一个色氨酸残基对于形成正常的bR570发色团是必不可少的。然而,在Trp-86突变体的bR----K和bR----M差光谱中,发现先前归因于bR----K光反应期间色氨酸残基扰动的742-cm-1负峰不存在。在此基础上,我们得出结论,在bR----K光反应期间,Trp-86的结构或环境发生了改变。所有其他Trp----Phe突变体都表现出这个波段,尽管其频率在Trp-189----Phe突变体中发生了改变。此外,相对于其他突变体,Trp-182----Phe突变体表现出正常光产物的形成大大减少,以及表明存在其他发色团构象的峰。讨论了一个bR模型,其中Trp-86、Trp-182和Trp-189构成视网膜结合口袋的一部分。这些色氨酸基团的一个可能功能是提供防止发色团在C13 = C14双键以外发生光异构化所需的结构约束。

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Vibrational spectroscopy of bacteriorhodopsin mutants: chromophore isomerization perturbs tryptophan-86.细菌视紫红质突变体的振动光谱:发色团异构化扰动色氨酸-86。
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