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Evidence of chemical exchange in recombinant Major Urinary Protein and quenching thereof upon pheromone binding.

Journal of biomolecular NMR (2007-03-08)
Chiara Perazzolo, Mariachiara Verde, Steve W Homans, Geoffrey Bodenhausen
RÉSUMÉ

The internal dynamics of recombinant Major Urinary Protein (rMUP) have been investigated by monitoring transverse nitrogen-15 relaxation using multiple-echo Carr-Purcell-Meiboom-Gill (CPMG) experiments. While the ligand-free protein (APO-rMUP) features extensive evidence of motions on the milliseconds time scale, the complex with 2-methoxy-3-isobutylpyrazine (HOLO-rMUP) appears to be much less mobile on this time scale. At 308 K, exchange rates k (ex) = 500-2000 s(-1) were typically observed in APO-rMUP for residues located adjacent to a beta-turn comprising residues 83-87. These residues occlude an entry to the binding pocket and have been proposed to be a portal for ligand entry in other members of the lipocalin family, such as the retinol binding protein and the human fatty-acid binding protein. Exchange rates and populations are largely uncorrelated, suggesting local 'breathing' motions rather than a concerted global conformational change.

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Sigma-Aldrich
2-Isobutyl-3-méthoxypyrazine, ≥99%, FG
Supelco
2-Isobutyl-3-methoxypyrazine solution, certified reference material
Sigma-Aldrich
2-Isobutyl-3-méthoxypyrazine, 99%