Abstract
The notable three oxygen stacking that occurs upon binding of ribonucleoside substrate and phosphate nucleophile by human purine nucleoside phosphorylase (hPNP) enables the coupling of protein dynamic modes to compress this stack, squeezing the ribosyl O4′ between ribosyl O5′ and the nuclophilic OP. Created primarily by the motion of active site residue H257, this compression dynamically lowers the barrier height for N9-C1′ ribosidic bond cleavage by as much as 20%. As such, this compression constitutes a protein promoting vibration (PPV) (S. Nuñez et al.). Presently, we demonstrate charge fluctuations in the ribose and purine components of the ribonucleoside substrate, as well as specifically across the N9-C1′ ribosidic bond, that are correlated with the PPV and can explain the decrease in reaction barrier height due to their facilitating cleavage of the ribosidic bond. hPNP apparently employs protein dynamics to push electrons, a finding that suggests that this coupling may be found more generally in enzymes that catalyze substitution and elimination reactions.
Original language | English (US) |
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Pages (from-to) | 501-509 |
Number of pages | 9 |
Journal | Journal of Theoretical and Computational Chemistry |
Volume | 3 |
Issue number | 4 |
DOIs | |
State | Published - Dec 2004 |
Keywords
- Catalysis
- Mechanism
- Protein dynamics
ASJC Scopus subject areas
- Computer Science Applications
- Physical and Theoretical Chemistry
- Computational Theory and Mathematics