AI Article Synopsis

  • - The B3 FEZ-1 beta-lactamase enzyme from Fluoribacter (Legionella) gormanii breaks down various antibiotics, including penicillins and carbapenems, and is dependent on zinc for its activity.
  • - Researchers created five specific mutants of FEZ-1 to study how changes to certain amino acids affect zinc and substrate binding, revealing important insights into the enzyme's functionality.
  • - The study found that some mutants altered the enzyme's effectiveness against certain antibiotics, with one mutant forming an inactive complex with hydrolyzed cephalosporins.

Article Abstract

The subclass B3 FEZ-1 beta-lactamase produced by Fluoribacter (Legionella) gormanii is a Zn(II)-containing enzyme that hydrolyzes the beta-lactam bond in penicillins, cephalosporins, and carbapenems. FEZ-1 has been extensively studied using kinetic, computational modeling and x-ray crystallography. In an effort to probe residues potentially involved in substrate binding and zinc binding, five site-directed mutants of FEZ-1 (H121A, Y156A, S221A, N225A, and Y228A) were prepared and characterized using metal analyses and steady state kinetics. The activity of H121A is dependent on zinc ion concentration. The H121A monozinc form is less active than the dizinc form, which exhibits an activity similar to that of the wild type enzyme. Tyr156 is not essential for binding and hydrolysis of the substrate. Substitution of residues Ser221 and Asn225 modifies the substrate profile by selectively decreasing the activity against carbapenems. The Y228A mutant is inhibited by the product formed upon hydrolysis of cephalosporins. A covalent bond between the side chain of Cys200 and the hydrolyzed cephalosporins leads to the formation of an inactive and stable complex.

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Source
http://dx.doi.org/10.1074/jbc.M403671200DOI Listing

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