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膜蛋白内的一个离域质子结合位点。

A delocalized proton-binding site within a membrane protein.

作者信息

Wolf Steffen, Freier Erik, Gerwert Klaus

机构信息

Department of Biophysics, Chinese Academy of Sciences-Max-Planck-Gesellschaft Partner Institute for Computational Biology, Shanghai Institutes for Biological Sciences, Shanghai, P.R. China.

Department of Biophysics, University of Bochum, Bochum, Germany.

出版信息

Biophys J. 2014 Jul 1;107(1):174-84. doi: 10.1016/j.bpj.2014.05.019.

Abstract

The role of protein-bound water molecules in protein function and catalysis is an emerging topic. Here, we studied the solvation of an excess proton by protein-bound water molecules and the contribution of the surrounding amino acid residues at the proton release site of the membrane protein bacteriorhodopsin. It hosts an excess proton within a protein-bound water cluster, which is hydrogen bonded to several surrounding amino acids. Indicative of delocalization is a broad continuum absorbance experimentally observed by time-resolved Fourier transform infrared spectroscopy. In combination with site-directed mutagenesis, the involvement of several amino acids (especially Glu-194 and Glu-204) in the delocalization was elaborated. Details regarding the contributions of the glutamates and water molecules to the delocalization mode in biomolecular simulations are controversial. We carried out quantum mechanics/molecular mechanics (QM/MM) self-consistent charge density functional tight-binding simulations for all amino acids that have been experimentally shown to be involved in solvation of the excess proton, and systematically investigated the influence of the quantum box size. We compared calculated theoretical infrared spectra with experimental ones as a measure for the correct description of excess proton delocalization. A continuum absorbance can only be observed for small quantum boxes containing few amino acids and/or water molecules. Larger quantum boxes, including all experimentally shown involved amino acids, resulted in narrow absorbance bands, indicating protonation of a single binding site in contradiction to experimental results. We conclude that small quantum boxes seem to reproduce representative extreme cases of proton delocalization modes: proton delocalization only on water molecules or only between Glu-194 and Glu-204. Extending the experimental spectral region to lower wave numbers, a water-delocalized proton reproduces the observed continuum absorbance better than a glutamate-shared delocalized proton. However, a full agreement between QM simulations and experimental results on the delocalized excess proton will require a larger quantum box as well as more sophisticated QM/MM methods.

摘要

蛋白质结合水分子在蛋白质功能和催化中的作用是一个新兴的研究课题。在此,我们研究了蛋白质结合水分子对过量质子的溶剂化作用,以及膜蛋白细菌视紫红质质子释放位点周围氨基酸残基的贡献。它在一个与几个周围氨基酸形成氢键的蛋白质结合水簇中容纳一个过量质子。时间分辨傅里叶变换红外光谱实验观察到的宽连续吸收表明了质子的离域。结合定点诱变,阐述了几种氨基酸(特别是Glu-194和Glu-204)在离域中的作用。关于谷氨酸和水分子对生物分子模拟中离域模式贡献的细节存在争议。我们对所有经实验证明参与过量质子溶剂化的氨基酸进行了量子力学/分子力学(QM/MM)自洽电荷密度泛函紧束缚模拟,并系统地研究了量子盒大小的影响。我们将计算得到的理论红外光谱与实验光谱进行比较,以此作为对过量质子离域正确描述的一种度量。只有对于包含少量氨基酸和/或水分子的小量子盒才能观察到连续吸收。更大的量子盒,包括所有经实验证明参与的氨基酸,会导致吸收带变窄,这表明与实验结果相反,单个结合位点发生了质子化。我们得出结论,小量子盒似乎能重现质子离域模式的代表性极端情况:质子仅在水分子上离域或仅在Glu-194和Glu-204之间离域。将实验光谱区域扩展到更低波数,水离域质子比谷氨酸共享离域质子能更好地重现观察到的连续吸收。然而,要使QM模拟与关于离域过量质子的实验结果完全一致,将需要更大的量子盒以及更复杂的QM/MM方法。

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