IDENTIFICATION OF THE BARSTAR BINDING-SITE OF BARNASE BY NMR-SPECTROSCOPY AND HYDROGEN-DEUTERIUM EXCHANGE

The extracellular ribonuclease from Bacillus amyloliquifaciens, barnase, forms a tightly-bound one-to-one complex with its intracellular inhibitor barstar. The barstar binding site on barnase was characterised by comparing the differences in the chemical shift and hydrogen-deuterium exchange rates between free and bound barnase. Chemical shift assignments of barnase in the complex with barstar were determined from 3D NOESY-HMQC and TOCSY-HMQC spectra of a complex that had been prepared with uniformly N-15-labelled barnase and unlabelled barstar. Hydrogen exchange rates were obtained from an analysis of a series of [N-15]HMQC spectra of a sample prepared in the same manner exchanged into D2O. The largest changes in either chemical shift or hydrogen-deuterium exchange rate are observed for residues located in the active-site and substrate binding loops indicating that barstar inhibits barnase activity by sterically blocking the active site.