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一种用不可异构化的13-反式视黄醛衍生物重构的细菌视紫红质类似物表现出光不敏感性。

A bacteriorhodopsin analog reconstituted with a nonisomerizable 13-trans retinal derivative displays light insensitivity.

作者信息

Bhattacharya S, Marti T, Otto H, Heyn M P, Khorana H G

机构信息

Department of Biology, Massachusetts Institute of Technology, Cambridge 02139.

出版信息

J Biol Chem. 1992 Apr 5;267(10):6757-62.

PMID:1551884
Abstract

With the aim of preparing a light-insensitive bacteriorhodopsin-like pigment, bacterio-opsin expressed in Escherichia coli was treated in phospholipid-detergent micelles with the retinal analog II, in which the C13-C14 trans-double bond cannot isomerize due to inclusion in a cyclopentene ring. The formation of a complex with a fine structure (lambda max, 439 nm) was first observed. This partially converted over a period of 12 days to a bacteriorhodopsin-like chromophore (ebR-II) with lambda max, 555 nm. An identical behavior has been observed previously upon reconstitution of bleached purple membrane with the analog II. Purification by gel filtration gave pure ebR-II with lambda max, 558 nm, similar to that of light-adapted bacterio-opsin reconstituted with all-trans retinal (ebR-I). Spectrophotometric titration of ebR-II as a function of pH showed that the purple to blue transition of bacteriorhodopsin at acidic pH was altered, and the apparent pKa of Schiff base deprotonation at alkaline pH was lowered by 2.4 units, relative to that of ebR-I. ebR-II showed no light-dark adaptation, no proton pumping, and no intermediates characteristic of the bacteriorhodopsin photocycle. In addition, the rates of reaction with hydroxylamine in the dark and in the light were similar. These results show, as expected, that isomerization of the C13-C14 double bond is required for bacteriorhodopsin function and that prevention of this isomerization confers light insensitivity.

摘要

为了制备一种对光不敏感的类细菌视紫红质色素,在磷脂 - 去污剂胶束中用视黄醛类似物II处理在大肠杆菌中表达的细菌视蛋白,其中由于包含在环戊烯环中,C13 - C14反式双键不能异构化。首次观察到形成了具有精细结构(最大吸收波长为439 nm)的复合物。这种复合物在12天的时间里部分转化为一种类细菌视紫红质发色团(ebR - II),其最大吸收波长为555 nm。先前在用类似物II重建漂白的紫膜时也观察到了相同的行为。通过凝胶过滤纯化得到了最大吸收波长为558 nm的纯ebR - II,类似于用全反式视黄醛重建的光适应细菌视蛋白(ebR - I)。ebR - II的分光光度滴定作为pH的函数表明,细菌视紫红质在酸性pH下从紫色到蓝色的转变发生了改变,并且相对于ebR - I,在碱性pH下席夫碱去质子化的表观pKa降低了2.4个单位。ebR - II没有明暗适应,没有质子泵浦,也没有细菌视紫红质光循环特有的中间体。此外,在黑暗和光照下与羟胺反应的速率相似。这些结果正如预期的那样表明,细菌视紫红质功能需要C13 - C14双键的异构化,并且防止这种异构化赋予了光不敏感性。

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