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用光域超快拉曼光谱探测光致变色黄色蛋白中光感应的早期阶段。

Probing the early stages of photoreception in photoactive yellow protein with ultrafast time-domain Raman spectroscopy.

机构信息

Molecular Spectroscopy Laboratory, RIKEN, 2-1 Hirosawa, Wako 351-0198, Japan.

Ultrafast Spectroscopy Research Team, RIKEN Center for Advanced Photonics (RAP), 2-1 Hirosawa, Wako 351-0198, Japan.

出版信息

Nat Chem. 2017 Jul;9(7):660-666. doi: 10.1038/nchem.2717. Epub 2017 Feb 6.

Abstract

Unveiling the nuclear motions of photoreceptor proteins in action is a crucial goal in protein science in order to understand their elaborate mechanisms and how they achieve optimal selectivity and efficiency. Previous studies have provided detailed information on the structures of intermediates that appear during the later stages (>ns) of such photoreception cycles, yet the initial events immediately after photoabsorption remain unclear because of experimental challenges in monitoring nuclear rearrangements on ultrafast timescales, including protein-specific low-frequency motions. Using time-domain Raman probing with sub-7-fs pulses, we obtain snapshot vibrational spectra of photoactive yellow protein and a mutant with high sensitivity, providing insights into the key responses that drive photoreception. Our data show a drastic intensity drop of the excited-state marker band at 135 cm within a few hundred femtoseconds, suggesting a rapid weakening of the hydrogen bond that anchors the chromophore. We also track formation of the first ground-state intermediate over the first few picoseconds and fully characterize its vibrational structure, revealing a substantially-twisted cis conformation.

摘要

揭示光感受器蛋白在作用中的核运动是蛋白质科学中的一个关键目标,以便了解它们复杂的机制以及它们如何实现最佳的选择性和效率。先前的研究已经提供了关于在这些光受体循环的后期(>ns)阶段出现的中间体结构的详细信息,但由于在超快时间尺度上监测核重排的实验挑战,包括与蛋白质特异性低频运动相关的挑战,光吸收后立即发生的初始事件仍然不清楚。我们使用具有亚 7 飞秒脉冲的时域拉曼探测技术,获得了光活性黄色蛋白及其突变体的高灵敏度快照振动光谱,为驱动光受体的关键响应提供了深入了解。我们的数据表明,在几百飞秒内,位于 135cm 的激发态标记带的强度急剧下降,这表明固定发色团的氢键迅速减弱。我们还跟踪了最初的基态中间体在最初的几个皮秒内的形成,并完全表征了其振动结构,揭示了其显著扭曲的顺式构象。

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