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通过光谱和 X 射线溶液散射研究测定光致变色黄色蛋白中发色团去除诱导的构象变化。

Chromophore-Removal-Induced Conformational Change in Photoactive Yellow Protein Determined through Spectroscopic and X-ray Solution Scattering Studies.

机构信息

Department of Chemistry and KI for the BioCentury , Korea Advanced Institute of Science and Technology (KAIST) , Daejeon 34141 , Republic of Korea.

Center for Nanomaterials and Chemical Reactions , Institute for Basic Science (IBS) , Daejeon 34141 , Republic of Korea.

出版信息

J Phys Chem B. 2018 Apr 26;122(16):4513-4520. doi: 10.1021/acs.jpcb.8b01768. Epub 2018 Apr 17.

DOI:10.1021/acs.jpcb.8b01768
PMID:29648836
Abstract

Photoactive yellow protein (PYP) induces negative phototaxis in Halorhodospira halophila via photoactivation triggered by light-mediated chromophore isomerization. Chromophore isomerization proceeds via a volume-conserving isomerization mechanism due to the hydrogen-bond network and steric constraints inside the protein, and causes significant conformational changes accompanied by N-terminal protrusion. However, it is unclear how the structural change of the chromophore affects the remote N-terminal domain. To understand photocycle-related structural changes, we investigated the structural aspect of chromophore removal in PYP because it possesses a disrupted hydrogen-bond network similar to that in photocycle intermediates. A comparison of the structural aspects with those observed in the photocycle would give a clue related to the structural change mechanism in the photocycle Chromophore removal effects were assessed via UV-vis spectroscopy, circular dichroism, and X-ray solution scattering. Molecular shape reconstruction and an experiment-restrained rigid-body molecular dynamics simulation based on the scattering data were performed to determine protein shape, size, and conformational changes upon PYP bleaching. Data show that chromophore removal disrupted the holo-PYP structure, resulting in a small N-terminal protrusion, but the extent of conformational changes was markedly less than those in the photocycle. This indicates that disruption of the hydrogen-bond network alone in bleached PYP does not induce the large conformational change observed in the photocycle, which thus must result from the organized structural transition around the chromophore triggered by chromophore photoisomerization along with disruption of the hydrogen-bond network between the chromophore and the PYP core.

摘要

光激活黄色蛋白(PYP)通过光介导的发色团异构化触发的光激活诱导盐沼盐杆菌产生负趋光性。由于蛋白质内部的氢键网络和空间限制,发色团异构化通过体积守恒的异构化机制进行,导致伴随 N 端突出的显著构象变化。然而,发色团结构变化如何影响远程 N 端结构域尚不清楚。为了了解光循环相关的结构变化,我们研究了 PYP 中发色团去除的结构方面,因为它具有类似于光循环中间体的破坏氢键网络。与光循环中观察到的结构方面进行比较将为光循环中的结构变化机制提供线索。通过紫外可见光谱、圆二色性和 X 射线溶液散射评估了发色团去除的效果。进行了分子形状重建和基于散射数据的实验约束刚体分子动力学模拟,以确定 PYP 漂白时的蛋白质形状、大小和构象变化。数据表明,发色团去除破坏了全酶 PYP 的结构,导致 N 端小突起,但构象变化的程度明显小于光循环中的变化。这表明,在漂白的 PYP 中仅破坏氢键网络不会引起光循环中观察到的大构象变化,因此这种变化必须是由发色团光异构化引发的围绕发色团的有组织的结构转变引起的,同时伴随着发色团和 PYP 核心之间氢键网络的破坏。

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