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细菌叶绿素激子在捕光复合体LH2中的溶剂化效应。

Solvation effect of bacteriochlorophyll excitons in light-harvesting complex LH2.

作者信息

Urboniene V, Vrublevskaja O, Trinkunas G, Gall A, Robert B, Valkunas L

机构信息

Department of General Physics and Spectroscopy, Vilnius University, Vilnius, Lithuania.

出版信息

Biophys J. 2007 Sep 15;93(6):2188-98. doi: 10.1529/biophysj.106.103093. Epub 2007 May 18.

Abstract

We have characterized the influence of the protein environment on the spectral properties of the bacteriochlorophyll (Bchl) molecules of the peripheral light-harvesting (or LH2) complex from Rhodobacter sphaeroides. The spectral density functions of the pigments responsible for the 800 and 850 nm electronic transitions were determined from the temperature dependence of the Bchl absorption spectra in different environments (detergent micelles and native membranes). The spectral density function is virtually independent of the hydrophobic support that the protein experiences. The reorganization energy for the B850 Bchls is 220 cm(-1), which is almost twice that of the B800 Bchls, and its Huang-Rhys factor reaches 8.4. Around the transition point temperature, and at higher temperatures, both the static spectral inhomogeneity and the resonance interactions become temperature-dependent. The inhomogeneous distribution function of the transitions exhibits less temperature dependence when LH2 is embedded in membranes, suggesting that the lipid phase protects the protein. However, the temperature dependence of the fluorescence spectra of LH2 cannot be fitted using the same parameters determined from the analysis of the absorption spectra. Correct fitting requires the lowest exciton states to be additionally shifted to the red, suggesting the reorganization of the exciton spectrum.

摘要

我们已经表征了蛋白质环境对球形红杆菌外周光捕获(或LH2)复合物中细菌叶绿素(Bchl)分子光谱特性的影响。通过不同环境(去污剂胶束和天然膜)中Bchl吸收光谱的温度依赖性,确定了负责800和850 nm电子跃迁的色素的光谱密度函数。光谱密度函数实际上与蛋白质所处的疏水支持物无关。B850 Bchls的重组能为220 cm(-1),几乎是B800 Bchls的两倍,其黄-里斯因子达到8.4。在转变点温度附近及更高温度下,静态光谱不均匀性和共振相互作用均变得与温度相关。当LH2嵌入膜中时,跃迁的不均匀分布函数对温度的依赖性较小,这表明脂质相保护了蛋白质。然而,LH2荧光光谱的温度依赖性不能用从吸收光谱分析确定的相同参数来拟合。正确的拟合需要最低激子态额外向红光方向移动,这表明激子光谱发生了重组。

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