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光活性黄色蛋白发色团类似物的超快光诱导响应

Ultrafast light-induced response of photoactive yellow protein chromophore analogues.

作者信息

Espagne Agathe, Paik Daniel H, Changenet-Barret Pascale, Plaza Pascal, Martin Monique M, Zewail Ahmed H

机构信息

UMR CNRS-ENS 8640 PASTEUR, Département de Chimie, Ecole Normale Supérieure, 24 rue Lhomond, 75005, Paris, France.

出版信息

Photochem Photobiol Sci. 2007 Jul;6(7):780-7. doi: 10.1039/b700927e. Epub 2007 Apr 18.

DOI:10.1039/b700927e
PMID:17609772
Abstract

The fluorescence decays of several analogues of the photoactive yellow protein (PYP) chromophore in aqueous solution have been measured by femtosecond fluorescence up-conversion and the corresponding time-resolved fluorescence spectra have been reconstructed. The native chromophore of PYP is a thioester derivative of p-coumaric acid in its trans deprotonated form. Fluorescence kinetics are reported for a thioester phenyl analogue and for two analogues where the thioester group has been changed to amide and carboxylate groups. The kinetics are compared to those we previously reported for the analogues bearing ketone and ester groups. The fluorescence decays of the full series are found to lie in the 1-10 ps range depending on the electron-acceptor character of the substituent, in good agreement with the excited-state relaxation kinetics extracted from transient absorption measurements. Steady-state photolysis is also examined and found to depend strongly on the nature of the substituent. While it has been shown that the ultrafast light-induced response of the chromophore in PYP is controlled by the properties of the protein nanospace, the present results demonstrate that, in solution, the relaxation dynamics and pathway of the chromophore is controlled by its electron donor-acceptor structure: structures of stronger electron donor-acceptor character lead to faster decays and less photoisomerisation.

摘要

通过飞秒荧光上转换测量了光活性黄色蛋白(PYP)发色团的几种类似物在水溶液中的荧光衰减,并重建了相应的时间分辨荧光光谱。PYP的天然发色团是反式去质子化形式的对香豆酸硫酯衍生物。报道了硫酯苯基类似物以及硫酯基团已变为酰胺和羧酸酯基团的两种类似物的荧光动力学。将这些动力学与我们之前报道的带有酮和酯基团的类似物的动力学进行了比较。发现整个系列的荧光衰减范围在1 - 10皮秒之间,这取决于取代基的电子受体特性,与从瞬态吸收测量中提取的激发态弛豫动力学非常吻合。还研究了稳态光解,发现其强烈依赖于取代基的性质。虽然已经表明PYP中发色团的超快光诱导响应受蛋白质纳米空间性质的控制,但目前的结果表明,在溶液中,发色团的弛豫动力学和途径受其电子供体 - 受体结构控制:具有更强电子供体 - 受体特性的结构导致更快的衰减和更少的光异构化。

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Ultrafast light-induced response of photoactive yellow protein chromophore analogues.光活性黄色蛋白发色团类似物的超快光诱导响应
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Time-resolved single tryptophan fluorescence in photoactive yellow protein monitors changes in the chromophore structure during the photocycle via energy transfer.光活性黄色蛋白中时间分辨的单个色氨酸荧光通过能量转移监测光循环过程中发色团结构的变化。
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Strong hydrogen bond between glutamic acid 46 and chromophore leads to the intermediate spectral form and excited state proton transfer in the Y42F mutant of the photoreceptor photoactive yellow protein.感光蛋白光活性黄色蛋白的Y42F突变体中,谷氨酸46与发色团之间强烈的氢键导致了中间光谱形式和激发态质子转移。
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Distinguishing chromophore structures of photocycle intermediates of the photoreceptor PYP by transient fluorescence and energy transfer.通过瞬态荧光和能量转移区分光感受器PYP光循环中间体的发色团结构
J Phys Chem B. 2008 Jul 31;112(30):9118-25. doi: 10.1021/jp801174z. Epub 2008 Jul 8.

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Photoactive Yellow Protein Chromophore Photoisomerizes around a Single Bond if the Double Bond Is Locked.如果双键被锁定,光活性黄色蛋白发色团会围绕单键发生光异构化。
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Volume-conserving trans-cis isomerization pathways in photoactive yellow protein visualized by picosecond X-ray crystallography.
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Controlling the photoreactivity of the photoactive yellow protein chromophore by substituting at the p-coumaric acid group.通过取代对香豆酸基团来控制光致变色黄色蛋白发色团的光反应性。
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