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蛋白质波动通过一氧化碳和叠氮化物探针振动的受激红外回声来检测。

Protein fluctuations are sensed by stimulated infrared echoes of the vibrations of carbon monoxide and azide probes.

作者信息

Lim M, Hamm P, Hochstrasser R M

机构信息

Department of Chemistry, University of Pennsylvania, Philadelphia, PA 19104, USA.

出版信息

Proc Natl Acad Sci U S A. 1998 Dec 22;95(26):15315-20. doi: 10.1073/pnas.95.26.15315.

Abstract

The correlation functions of the fluctuations of vibrational frequencies of azide ions and carbon monoxide in proteins are determined directly from stimulated photon echoes generated with femtosecond infrared pulses. The asymmetric stretching vibration of azide bound to carbonic anhydrase II exhibits a pronounced evolution of its vibrational frequency distribution on the time scale of a few picoseconds, which is attributed to modifications of the ligand structure through interactions with the nearby Thr-199. When azide is bound in hemoglobin, a more complex evolution of the protein structure is required to interchange the different ligand configurations, as evidenced by the much slower relaxation of the frequency distribution in this case. The time evolution of the distribution of frequencies of carbon monoxide bound in hemoglobin occurs on the approximately 10-ps time scale and is very nonexponential. The correlation functions of the frequency fluctuations determine the evolution of the protein structure local to the probe and the extent to which the probe can navigate those parts of the energy landscape where the structural configurations are able to modify the local potential energy function of the probe.

摘要

通过飞秒红外脉冲产生的受激光子回波,直接测定了蛋白质中叠氮离子和一氧化碳振动频率涨落的关联函数。与碳酸酐酶II结合的叠氮的不对称伸缩振动,在几皮秒的时间尺度上,其振动频率分布呈现出明显的演化,这归因于通过与附近的苏氨酸-199相互作用对配体结构的修饰。当叠氮结合在血红蛋白中时,需要更复杂的蛋白质结构演化来互换不同的配体构型,在这种情况下频率分布的弛豫要慢得多就证明了这一点。结合在血红蛋白中的一氧化碳频率分布的时间演化发生在大约10皮秒的时间尺度上,并且非常非指数化。频率涨落的关联函数决定了探针局部蛋白质结构的演化,以及探针能够在能量景观中那些结构构型能够修改探针局部势能函数的部分中导航的程度。

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