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Protein Field Effect on the Dark State of 11-cis Retinal in Rhodopsin by Quantum Monte Carlo/Molecular Mechanics

机译:对暗态蛋白质场效应11-顺式视网膜视紫红质的量子蒙特卡罗/分子力学

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摘要

The accurate determination of the geometrical details of the dark state of 11-cis retinal in rhodopsin represents a fundamental step for the rationalization of the protein role in the optical spectral tuning in the vision mechanism. We have calculated geometries of the full retinal protonated Schiff base chromophore in the gas phase and in the protein environment using the correlated variational Monte Carlo method. The bond length alternation of the conjugated carbon chain of the chromophore in the gas phase shows a significant reduction when moving from the β-ionone ring to the nitrogen, whereas, as expected, the protein environment reduces the electronic conjugation. The proposed dark state structure is fully compatible with solid-state NMR data reported by Carravetta et al. [J. Am. Chem. Soc. >2004, 126, 3948–3953]. TDDFT/B3LYP calculations on such geometries show a blue opsin shift of 0.28 and 0.24 eV induced by the protein for S1 and S2 states, consistently with literature spectroscopic data. The effect of the geometrical distortion alone is a red shift of 0.21 and 0.16 eV with respect to the optimized gas phase chromophore. Our results open new perspectives for the study of the properties of chromophores in their biological environment using correlated methods.
机译:视紫红质中11-顺式视网膜黑暗状态的几何细节的准确确定代表了合理化视觉机制中光谱调节中蛋白质作用的基本步骤。我们已经使用相关的变分蒙特卡罗方法计算了气相和蛋白质环境中全视网膜质子化席夫碱生色团的几何形状。当从β-紫罗兰酮环移到氮原子时,气相中发色团共轭碳链的键长变化显示出明显的减少,而正如所预期的,蛋白质环境减少了电子共轭。提出的暗态结构与Carravetta等报道的固态NMR数据完全兼容。 [J.上午。化学Soc。 > 2004 ,第126页,3948–3953]。在此类几何结构上的TDDFT / B3LYP计算显示,蛋白质针对S1和S2状态引起的蓝色视蛋白移位为0.28和0.24 eV,与文献光谱数据一致。相对于优化的气相生色团,仅几何畸变的影响就是0.21和0.16 eV的红移。我们的结果为使用相关方法研究生色团在其生物环境中的性质开辟了新的前景。

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