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Femtochemistry in enzyme catalysis: DNA photolyase

Journal

CELL BIOCHEMISTRY AND BIOPHYSICS
Volume 48, Issue 1, Pages 32-44

Publisher

HUMANA PRESS INC
DOI: 10.1007/s12013-007-0034-5

Keywords

femtochemistry; enzyme catalysis; DNA photolyase; solvation dynamics; photoinitiation; resonance energy transfer (RET); photoreduction; electron transfer (ET); photorepair; cyclobutane pyrimidine dimer (CPD); DNA repair

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Photolyase uses light energy to split UV-induced cyclobutane pyrimidine dimers in damaged DNA. This photoenzyme encompasses a series of elementary dynamical processes during repair function from early photoinitiation by a photoantenna molecule to enhance repair efficiency, to in vitro photoreduction through aromatic residues to reconvert the cofactor to the active form, and to final photorepair to fix damaged DNA. The corresponding series of dynamics include resonance energy transfer, intraprotein electron transfer, and intermolecular electron transfer, bond breaking-making rearrangements and back electron return, respectively. We review here our recent direct studies of these dynamical processes in real time, which showed that all these elementary reactions in the enzyme occur within subnanosecond timescale. Active-site solvation was observed to play a critical role in the continuous modulation of catalytic reactions. As a model system for enzyme catalysis, we isolated the enzyme-substrate complex in the transition-state region and mapped out the entire evolution of unmasked catalytic reactions of DNA repair. These observed synergistic motions in the active site reveal a perfect correlation of structural integrity and dynamical locality to ensure maximum repair efficiency on the ultrafast time scale.

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