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首页> 外文期刊>Frontiers in Molecular Biosciences >The primary photoreaction of channelrhodopsin-1: wavelength dependent photoreactions induced by ground-state heterogeneity
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The primary photoreaction of channelrhodopsin-1: wavelength dependent photoreactions induced by ground-state heterogeneity

机译:视紫红质-1的主要光反应:基态异质性诱导的波长依赖性光反应

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The primary photodynamics of channelrhodopsin-1 from Chlamydomonas augustae (CaChR1) was investigated by VIS-pump supercontinuum probe experiments from femtoseconds to 100 picoseconds. In contrast to reported experiments on channelrhodopsin-2 from Chlamydomonas reinhardtii (CrChR2), we found a clear dependence of the photoreaction dynamics on varying the excitation wavelength. Upon excitation at 500 nm and at 550 nm we detected different bleaching bands, andspectrally distinct photoproduct absorptions in the first picoseconds. We assign the former to the ground-state heterogeneity of a mixture of 13-cis and all-trans retinal maximally absorbing around 480 nm and 540 nm, respectively. At 550 nm, all-trans retinal of the ground state is almost exclusively excited. Here, we found a fast all-trans to 13-cis isomerization process to a hot and spectrally broad P1 photoproduct with a time constant of (100±50) fs, followed by photoproduct relaxation with time constants of (500±100) fs and (5±1) ps. The remaining fraction relaxes back to the parent ground state with time constants of (500±100) fs and (5±1) ps. Upon excitation at 500 nm a mixture of both chromophore conformations is excited, resulting in overlapping reaction dynamics with additional time constants of <300 fs, (1.8±0.3) ps and (90±25) ps. A new photoproduct Q is formed absorbing at around 600 nm. Strong coherent oscillatory signals were found pertaining up to several picoseconds. We determined low frequency modes around 200 cm-1, similar to those reported for bacteriorhodopsin.
机译:通过飞秒至100皮秒的VIS-pump超连续谱探针实验研究了来自衣藻衣藻(CaChR1)的Channelrhodopsin-1的主要光动力学。与报道的对莱茵衣藻(ChChyydomonas reinhardtii)(CrChR2)的channelrhodopsin-2进行的实验相反,我们发现光反应动力学对激发波长的变化有明显的依赖性。在500 nm和550 nm激发后,我们在最初的皮秒内检测到了不同的漂白带和光谱不同的光产物吸收。我们将前者分配给最大吸收约480 nm和540 nm的13-顺式和全反式视网膜混合物的基态异质性。在550 nm处,基态的全反式视网膜几乎全部被激发。在这里,我们发现了一个快速的全反式至13-顺式异构化过程,该过程是热的且光谱宽广的P1光产物,其时间常数为(100±50)fs,然后是光产物弛豫,其时间常数为(500±100)fs和(5±1)ps。其余部分以(500±100)fs和(5±1)ps的时间常数弛豫回母体基态。在500 nm激发后,两种生色团构象的混合物都被激发,从而产生了重叠的反应动力学,并具有<300 fs,(1.8±0.3)ps和(90±25)ps的附加时间常数。形成新的光产物Q,其在约600nm处吸收。发现强相干振荡信号长达数皮秒。我们确定了200 cm-1附近的低频模式,这与细菌视紫红质的报道相似。

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