Three factors that modulate the activity of class D β-lactamases and interfere with the post-translational carboxylation of Lys70

Author:

Vercheval Lionel1,Bauvois Cédric2,di Paolo Alexandre3,Borel Franck4,Ferrer Jean-Luc4,Sauvage Eric5,Matagne André3,Frère Jean-Marie3,Charlier Paulette5,Galleni Moreno1,Kerff Frédéric5

Affiliation:

1. Laboratory of Biological Macromolecules, Centre for Protein Engineering, Institut de Chimie B6a, University of Liège, Liège 4000, Belgium

2. Cristallographie des protéines, Institut de Recherches Microbiologiques J.-M. Wiame (IRMW), Bruxelles 1070, Belgium

3. Laboratory of Enzymology and Protein Folding, Centre for Protein Engineering, Institut de Chimie B6a, University of Liège, Liège 4000, Belgium

4. Laboratoire de Cristallographie et Cristallogenèse des Protéines, Institut de Biologie Structurale J-P. Ebel, CEA/CNRS/UJ.F, Grenoble 38027, France

5. Laboratory of Protein Crystallography, Centre for Protein Engineering, Institut de Chimie B6a, University of Liège, Liège 4000, Belgium

Abstract

The activity of class D β-lactamases is dependent on Lys70 carboxylation in the active site. Structural, kinetic and affinity studies show that this post-translational modification can be affected by the presence of a poor substrate such as moxalactam but also by the V117T substitution. Val117 is a strictly conserved hydrophobic residue located in the active site. In addition, inhibition of class D β-lactamases by chloride ions is due to a competition between the side chain carboxylate of the modified Lys70 and chloride ions. Determination of the individual kinetic constants shows that the deacylation of the acyl–enzyme is the rate-limiting step for the wild-type OXA-10 β-lactamase.

Publisher

Portland Press Ltd.

Subject

Cell Biology,Molecular Biology,Biochemistry

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