Literature DB >> 11567101

On the involvement of electron transfer reactions in the fluorescence decay kinetics heterogeneity of proteins.

A Ababou1, E Bombarda.   

Abstract

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.

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Year:  2001        PMID: 11567101      PMCID: PMC2374218          DOI: 10.1110/ps.05501

Source DB:  PubMed          Journal:  Protein Sci        ISSN: 0961-8368            Impact factor:   6.725


  38 in total

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8.  Time-resolved fluorescence spectra of tryptophan in monomeric glucagon.

Authors:  S A Cockle; A G Szabo
Journal:  Photochem Photobiol       Date:  1981-07       Impact factor: 3.421

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Authors:  K J Willis; A G Szabo
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  11 in total

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8.  Tryptophan conformations associated with partial unfolding in ribonuclease T1.

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9.  Tryptophan environment and functional characterization of a kinetically stable serine protease containing a polyproline II fold.

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10.  Tryptophan properties in fluorescence and functional stability of plasminogen activator inhibitor 1.

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