Molecular Bases of Catalysis and ADP-Ribose Preference of Human Mn(2+)-Dependent ADP-Ribose/CDP-Alcohol Diphosphatase and Conversion by Mutagenesis to a Preferential Cyclic ADP-Ribose Phosphohydrolase

Among metallo-dependent phosphatases, ADP-ribose/CDP-alcohol diphosphatases form a protein family (ADPRibase-Mn-like) mainly restricted, in eukaryotes, to vertebrates and plants, with preferential expression, at least in rodents, in immune cells. Rat and zebrafish ADPRibase-Mn, the only biochemicall...

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Detalles Bibliográficos
Autores principales: Cabezas, Alicia, Ribeiro, João Meireles, Rodrigues, Joaquim Rui, López-Villamizar, Iralis, Fernández, Ascensión, Canales, José, Pinto, Rosa María, Costas, María Jesús, Cameselle, José Carlos
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4334965/
https://www.ncbi.nlm.nih.gov/pubmed/25692488
http://dx.doi.org/10.1371/journal.pone.0118680
Descripción
Sumario:Among metallo-dependent phosphatases, ADP-ribose/CDP-alcohol diphosphatases form a protein family (ADPRibase-Mn-like) mainly restricted, in eukaryotes, to vertebrates and plants, with preferential expression, at least in rodents, in immune cells. Rat and zebrafish ADPRibase-Mn, the only biochemically studied, are phosphohydrolases of ADP-ribose and, somewhat less efficiently, of CDP-alcohols and 2´,3´-cAMP. Furthermore, the rat but not the zebrafish enzyme displays a unique phosphohydrolytic activity on cyclic ADP-ribose. The molecular basis of such specificity is unknown. Human ADPRibase-Mn showed similar activities, including cyclic ADP-ribose phosphohydrolase, which seems thus common to mammalian ADPRibase-Mn. Substrate docking on a homology model of human ADPRibase-Mn suggested possible interactions of ADP-ribose with seven residues located, with one exception (Cys(253)), either within the metallo-dependent phosphatases signature (Gln(27), Asn(110), His(111)), or in unique structural regions of the ADPRibase-Mn family: s2s3 (Phe(37) and Arg(43)) and h7h8 (Phe(210)), around the active site entrance. Mutants were constructed, and kinetic parameters for ADP-ribose, CDP-choline, 2´,3´-cAMP and cyclic ADP-ribose were determined. Phe(37) was needed for ADP-ribose preference without catalytic effect, as indicated by the increased ADP-ribose K (m) and unchanged k (cat) of F37A-ADPRibase-Mn, while the K (m) values for the other substrates were little affected. Arg(43) was essential for catalysis as indicated by the drastic efficiency loss shown by R43A-ADPRibase-Mn. Unexpectedly, Cys(253) was hindering for cADPR phosphohydrolase, as indicated by the specific tenfold gain of efficiency of C253A-ADPRibase-Mn with cyclic ADP-ribose. This allowed the design of a triple mutant (F37A+L196F+C253A) for which cyclic ADP-ribose was the best substrate, with a catalytic efficiency of 3.5´10(4) M(-1)s(-1) versus 4´10(3) M(-1)s(-1) of the wild type.

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