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Photoinduced proton transfer inside an engineered green fluorescent protein: a stepwise-concerted-hybrid reaction

机译:在工程化绿色荧光蛋白内的光突出质子转移:逐步齐节 - 杂交反应

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Photoactivated proton transfer (PT) wire is responsible for the glow of green fluorescent protein (GFP), which is crucial for bioimaging and biomedicine. In this work, a new GFP-S65T/S205V double mutant is developed from wild-type GFP in which the PT wire is significantly modified. We implement femtosecond transient absorption (fs-TA) and femtosecond stimulated Raman spectroscopy (FSRS) to delineate the PT process in action. The excited state proton transfer proceeds on the similar to 110 ps timescale, which infers that the distance of one key link (water to T203) in the PT wire of GFP-S205V is shortened by the extra S65T mutation. The rise of an imidazolinone ring deformation mode at similar to 871 cm(-1) in FSRS further suggests that this PT reaction is in a concerted manner. A similar to 4 ps component prior to large-scale proton dissociation through the PT wire is also retrieved, indicative of some smallscale proton motions and heavy-atom rearrangement in the vicinity of the chromophore. Our work provides deep insights into the novel hybrid PT mechanism in engineered GFP and demonstrates the power of tunable FSRS methodology in tracking ultrafast photoreactions with the desirable structural specificity in physiological environments.
机译:PhotoCtivated质子转移(PT)丝负责绿色荧光蛋白(GFP)的辉光,这对于生物成像和生物医学是至关重要的。在这项工作中,从野生型GFP开发了一种新的GFP-S65T / S205V双突变体,其中PT线被显着修改。我们实施飞秒瞬态吸收(FS-TA)和飞秒刺激的拉曼光谱(FSRS)以划分PT过程的作用。激励状态质子转移在类似于110ps时间尺度上进行,其缩短了额外的S65T突变的PT线中的一个关键链路(水至T203)的距离。在FSRS中类似于871cm(-1)的咪唑啉环变形模式的升高进一步表明该PT反应以齐心的方式。还可以检索在大规模质子解离之前的类似于4 PS组分,指示发色团附近的一些小型质子运动和重原子重排。我们的工作在工程GFP中提供了深入的杂交PT机制,并展示了可调性FSRS方法的功率在跟踪超速度光反应,以生理环境中所需的结构特异性。

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