Purification and kinetic characterization of pickerel liver alcohol dehydrogenase with dual coenzyme specificity

Abstract

A major alcohol dehydrogenase isozyme that displays dual coenzyme specificity has been purified from pickerel liver by ion-exchange, gel filtration, and affinity chromatographic procedures. The purified enzyme is chromatographically and electrophoretically homogeneous. It is dimeric and possesses common physical properties shared by other liver alcohol dehydrogenases. Phosphorus-31 nuclear magnetic resonance spectroscopy demonstrates that NADP⁺ binds to two coenzyme sites of the pickerel enzyme. Steady-state kinetic studies suggest that pickerel liver alcohol dehydrogenase catalyzes NAD(P)⁺-linked ethanol oxidation via a random pathway. While the NADP⁺ reduction involves the formation of an abortive complex at high NADP⁺ concentrations, the NAD⁺ reduction at low NAD⁺ concentrations follows an ordered Bi-Bi mechanism with NAD⁺ being the leading reactant.Key words: purification, pickerel liver, alcohol dehydrogenase.