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细菌视紫红质突变体的振动光谱:脯氨酸-186与视黄叉发色团相互作用的证据。

Vibrational spectroscopy of bacteriorhodopsin mutants: evidence for the interaction of proline-186 with the retinylidene chromophore.

作者信息

Rothschild K J, He Y W, Mogi T, Marti T, Stern L J, Khorana H G

机构信息

Physics Department, Boston University, Massachusetts 02215.

出版信息

Biochemistry. 1990 Jun 26;29(25):5954-60. doi: 10.1021/bi00477a011.

DOI:10.1021/bi00477a011
PMID:2166567
Abstract

Fourier-transform infrared difference spectroscopy has been used to study the role of the three membrane-embedded proline residues, Pro-50, Pro-91, and Pro-186, in the structure and function of bacteriorhodopsin. All three prolines were replaced by alanine and glycine; in addition, Pro-186 was changed to valine. Difference spectra were recorded for the bR----K and bR----M photoreactions of each of these mutants and compared to those of wild-type bacteriorhodopsin. Only substitutions of Pro-186 caused significant perturbations in the frequency of the C = C and C - C stretching modes of the retinylidene chromophore. In addition, these substitutions reduced bands in the amide I and II region associated with secondary structural changes and altered signals assigned to the adjacent Tyr-185. Pro-186----Val caused the largest alterations, producing a second species similar to bR548 and nearly blocking chromophore isomerization at 78 K but not at 250 K. These results are consistent with a model of the retinal binding site in which Pro-186 and Tyr-185 are located in direct proximity to the chromophore and may be involved in linking chromophore isomerization to protein structural changes. Evidence is also found that Pro-50 may be structurally active during the bR----K transition and that substitution of this residue by glycine preserves the normal protein structural changes during the photocycle.

摘要

傅里叶变换红外差光谱已被用于研究细菌视紫红质结构和功能中三个膜嵌入脯氨酸残基(Pro-50、Pro-91和Pro-186)的作用。所有这三个脯氨酸都被丙氨酸和甘氨酸取代;此外,Pro-186被替换为缬氨酸。记录了这些突变体中每一个的bR→K和bR→M光反应的差光谱,并与野生型细菌视紫红质的差光谱进行比较。只有Pro-186的取代导致视黄醛发色团的C = C和C - C伸缩模式频率发生显著扰动。此外,这些取代减少了与二级结构变化相关的酰胺I和II区域的谱带,并改变了分配给相邻Tyr-185的信号。Pro-186→Val引起的变化最大,产生了一种类似于bR548的第二种物质,并且在78 K时几乎阻止了发色团异构化,但在250 K时没有。这些结果与视网膜结合位点的模型一致,其中Pro-186和Tyr-185直接靠近发色团,并且可能参与将发色团异构化与蛋白质结构变化联系起来。还发现证据表明Pro-50在bR→K转变过程中可能具有结构活性,并且用甘氨酸取代该残基可在光循环过程中保留正常的蛋白质结构变化。

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