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首页> 外文期刊>Protein Science: A Publication of the Protein Society >On the involvement of electron transfer reactions in the fluorescence decay kinetics heterogeneity of proteins.
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On the involvement of electron transfer reactions in the fluorescence decay kinetics heterogeneity of proteins.

机译:在电子转移反应参与荧光衰变动力学的蛋白质异质性上。

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Time-resolved fluorescence study of single tryptophan-containing proteins, nuclease, ribonuclease T1, protein G, glucagon, and mastoparan, has been carried out. Three different methods were used for the analysis of fluorescence decays: the iterative reconvolution method, as reviewed and developed in our laboratory, the maximum entropy method, and the recent method that we called "energy transfer" method. All the proteins show heterogeneous fluorescence kinetics (multiexponential decay). The origin of this heterogeneity is interpreted in terms of current theories of electron transfer process, which treat the electron transfer process as a radiationless transition. The theoretical electron transfer rate was calculated assuming the peptide bond carbonyl as the acceptor site. The good agreement between experimental and theoretical electron-transfer rates leads us to suggest that the electron-transfer process is the principal quenching mechanism of Trp fluorescence in proteins, resulting in heterogeneous fluorescence kinetics. Furthermore, the origin of apparent homogeneous fluorescence kinetics (monoexponential decay) in some proteins also can be explained on the basis of electron-transfer mechanism.
机译:已对单个含色氨酸的蛋白质,核酸酶,核糖核酸酶T1,蛋白质G,胰高血糖素和马索帕兰进行了时间分辨荧光研究。三种不同的方法用于分析荧光衰减:在我们的实验室中审查和开发的迭代再卷积方法,最大熵方法和最近称为“能量转移”方法的方法。所有的蛋白质都显示出异质的荧光动力学(多指数衰减)。异质性的起源是根据电子转移过程的当前理论来解释的,该理论将电子转移过程视为无辐射跃迁。假定肽键羰基为受体位点,计算理论电子传递速率。实验和理论电子传输速率之间的良好一致性使我们认为,电子传输过程是蛋白质中Trp荧光的主要猝灭机制,导致异质荧光动力学。此外,某些蛋白质的表观均一荧光动力学(单指数衰减)的起源也可以基于电子转移机理来解释。

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