Literature DB >> 11847281

High probability of disrupting a disulphide bridge mediated by an endogenous excited tryptophan residue.

Maria Teresa Neves-Petersen1, Zygmunt Gryczynski, Joseph Lakowicz, Peter Fojan, Shona Pedersen, Evamaria Petersen, Steffen Bjørn Petersen.   

Abstract

It is well known that ultraviolet (UV) radiation may reduce or even abolish the biological activity of proteins and enzymes. UV light, as a component of sunlight, is illuminating all light-exposed parts of living organisms, partly composed of proteins and enzymes. Although a considerable amount of empirical evidence for UV damage has been compiled, no deeper understanding of this important phenomenon has yet emerged. The present paper presents a detailed analysis of a classical example of UV-induced changes in three-dimensional structure and activity of a model enzyme, cutinase from Fusarium solani pisi. The effect of illumination duration and power has been investigated. A photon-induced mechanism responsible for structural and functional changes is proposed. Tryptophan excitation energy disrupts a neighboring disulphide bridge, which in turn leads to altered biological activity and stability. The loss of the disulphide bridge has a pronounced effect on the fluorescence quantum yield, which has been monitored as a function of illumination power. A general theoretical model for slow two-state chemical exchange is formulated, which allows for calculation of both the mean number of photons involved in the process and the ratio between the quantum yields of the two states. It is clear from the present data that the likelihood for UV damage of proteins is directly proportional to the intensity of the UV radiation. Consistent with the loss of the disulphide bridge, a complex pH-dependent change in the fluorescence lifetimes is observed. Earlier studies in this laboratory indicate that proteins are prone to such UV-induced radiation damage because tryptophan residues typically are located as next spatial neighbors to disulphide bridges. We believe that these observations may have far-reaching implications for protein stability and for assessing the true risks involved in increasing UV radiation loads on living organisms.

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Year:  2002        PMID: 11847281      PMCID: PMC2373466          DOI: 10.1110/ps.06002

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


  26 in total

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  28 in total

Review 1.  Spectroscopic studies of protein folding: linear and nonlinear methods.

Authors:  Arnaldo L Serrano; Matthias M Waegele; Feng Gai
Journal:  Protein Sci       Date:  2011-12-28       Impact factor: 6.725

2.  Photophysics, photochemistry and energetics of UV light induced disulphide bridge disruption in apo-α-lactalbumin.

Authors:  Manuel Correia; Maria Teresa Neves-Petersen; Antonietta Parracino; Ane Kold di Gennaro; Steffen B Petersen
Journal:  J Fluoresc       Date:  2011-10-14       Impact factor: 2.217

3.  Quenchers induce wavelength dependence on protein fluorescence lifetimes.

Authors:  Søren Klitgaard; M T Neves-Petersen; S B Petersen
Journal:  J Fluoresc       Date:  2006-06-23       Impact factor: 2.217

4.  Photophysics and photochemistry of horseradish peroxidase A2 upon ultraviolet illumination.

Authors:  Maria Teresa Neves-Petersen; Søren Klitgaard; Ana Sofia Leitão Carvalho; Steffen B Petersen; Maria Raquel Aires de Barros; Eduardo Pinho e Melo
Journal:  Biophys J       Date:  2006-12-22       Impact factor: 4.033

5.  Photonic activation of disulfide bridges achieves oriented protein immobilization on biosensor surfaces.

Authors:  Maria Teresa Neves-Petersen; Torben Snabe; Søren Klitgaard; Meg Duroux; Steffen B Petersen
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6.  The feasibility of coherent energy transfer in microtubules.

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Review 7.  Photo-Degradation of Therapeutic Proteins: Mechanistic Aspects.

Authors:  Christian Schöneich
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8.  Photodegradation Pathways of Protein Disulfides: Human Growth Hormone.

Authors:  Daniel Steinmann; Olivier Mozziconacci; Rupesh Bommana; John F Stobaugh; Y John Wang; Christian Schöneich
Journal:  Pharm Res       Date:  2017-09-18       Impact factor: 4.200

9.  Arraying prostate specific antigen PSA and Fab anti-PSA using light-assisted molecular immobilization technology.

Authors:  Antonietta Parracino; Maria Teresa Neves-Petersen; Ane Kold di Gennaro; Kim Pettersson; Timo Lövgren; Steffen B Petersen
Journal:  Protein Sci       Date:  2010-09       Impact factor: 6.725

10.  Flash photolysis of cutinase: identification and decay kinetics of transient intermediates formed upon UV excitation of aromatic residues.

Authors:  Maria Teresa Neves-Petersen; Søren Klitgaard; Torbjorn Pascher; Esben Skovsen; Tomas Polivka; Arkady Yartsev; Villly Sundström; Steffen B Petersen
Journal:  Biophys J       Date:  2009-07-08       Impact factor: 4.033

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