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A Catalytic Triad Is Responsible for Acid−Base Chemistry in the Ascaris suum NAD−Malic Enzyme^†

William E. Karsten,^‡ Dali Liu,^‡ G. S. Jagannatha Rao,^§ Ben G. Harris,^§ and Paul F. Cook*^‡

Department of Chemistry and Biochemistry, University of Oklahoma, 620 Parrington Oval, Norman, Oklahoma 73019, and Department of Molecular Biology and Immunology, University of North Texas Health Sciences Center, 3500 Camp Bowie Boulevard, Fort Worth, Texas 76107

Biochemistry, 2005, 44 (9), pp 3626–3635

DOI: 10.1021/bi047826o

Publication Date (Web): February 9, 2005

†

This work was supported by grants from the NSF (MCB 0091207) and the Oklahoma Center for the Advancement of Science and Technology (HR99-081) to P.F.C., grants from the NIH (AI24155, AI41552) and the Robert A. Welch Foundation (BK1309) to B.G.H., and funds for P.F.C. from an endowment to the University of Oklahoma to fund the Grayce B. Kerr Centennial Professorship in Biochemistry.

‡

University of Oklahoma.

University of North Texas Health Sciences Center.

Corresponding author. Tel: 405-325-4581. Fax: 405-325-7182. E-mail: pcook@chemdept.chem.ou.edu.

Abstract

The pH dependence of kinetic parameters of several active site mutants of the Ascaris suum NAD−malic enzyme was investigated to determine the role of amino acid residues likely involved in catalysis on the basis of three-dimensional structures of malic enzyme. Lysine 199 is positioned to act as the general base that accepts a proton from the 2-hydroxyl of malate during the hydride transfer step. The pH dependence of V/K_malate for the K199R mutant enzyme reveals a pK of 5.3 for an enzymatic group required to be unprotonated for activity and a second pK of 6.3 that leads to a 10-fold loss in activity above the pK of 6.3 to a new constant value up to pH 10. The V profile for K199R is pH independent from pH 5.5 to pH 10 and decreases below a pK of 4.9. Tyrosine 126 is positioned to act as the general acid that donates a proton to the enolpyruvate intermediate to form pyruvate. The pH dependence of V/K_malate for the Y126F mutant is qualitatively similar to K199R, with a requirement for a group to be unprotonated for activity with a pK of 5.6 and a partial activity loss of about 3-fold above a pK of 6.7 to a new constant value. The Y126F mutant enzyme is about 60000-fold less active than the wild-type enzyme. In contrast to K199R, the V rate profile for Y126F also shows a partial activity loss above pH 6.6. The wild-type pH profiles were reinvestigated in light of the discovery of the partial activity change for the mutant enzymes. The wild-type V/K_malate pH−rate profile exhibits the requirement for a group to be unprotonated for catalysis with a pK of 5.6 and also shows the partial activity loss above a pK of 6.4. The wild-type V pH−rate profile decreases below a pK of 5.2 and is pH independent from pH 5.5 to pH 10. Aspartate 294 is within hydrogen-bonding distance to K199 in the open and closed forms of malic enzyme. D294A is about 13000-fold less active than the wild-type enzyme, and the pH−rate profile for V/K_malate indicates the mutant is only active above pH 9. The data suggest that the pK present at about pH 5.6 in all of the pH profiles represents D294, and during catalysis D294 accepts a proton from K199 to allow K199 to act as a general base in the reaction. The pK for the general acid in the reaction is not observed, consistent with rapid tautomerization of enolpyruvate. No other ionizable group in the active site is likely responsible for the partial activity change observed in the pH profiles, and thus the group responsible is probably remote from the active site and the effect on activity is transmitted through the protein by a conformational change.