Asociación de los genes implicados en la codificaciónde proteina de unión a la penicilina 2a (pbp2a) conla expresión fenotípica de resistencia a la meticilinaen cepas De staphylococcus spp / Association of genes involved in coding binding protein penicillin 2a (PBP2a) with phenotypic expression of methicillin resistance in strains of Staphylococcus spp

Objetivo: Determinar si existe asociación entre genes implicados en la codificación de PBP2a con la expresión fenotípica de resistencia a meticilina en cepas de Staphylococcus spp. Diseño: Descriptivo Transversal. Metodologias: e determinó la resistencia y sensibilidad de 67 aislamientos, mediante pruebas fenotípicas (difusión en disco, concentración inhibitoriamínima CIM, producción de PBP2a y pruebas genotípicas para detectar los genes mecA y sus reguladores mecR1 y mecI por Reacción em Cadena de la Polimerasa (PCR). Resultados: De 9 cepas de S. aureus resistentes por difusión en disco solo 1 fue sensible por CIM. De 7 cepas resistentes por CIM, fueron sensibles por difusión en disco. Por el contrario las 7 cepas de Staphylococcus coagulasa negativo sensibles por difusión en disco fueron resistentespor CIM.En cuanto a la prueba de producción de PBP2a, los resultados fueron discordantes con la prueba de difusión en disco en 20..

Objective: Determining the association between genes involved in the codifi cation of Penicillin Binding Proteins 2A (PBP2A) with the phenotypic expression of methicillin resistance in Staphylococcus spp. Strains Design: Descriptive cross sectional Methodology: The sensitivity of 67 isolates was determined by means of a phenotypic test (disk diffusion, minimum inhibitory concentration CIM, production of PBP2a) and genotype tests to detect the mecA gene and its regulatory mecR1 and mecI by Polymerase Chain Reaction (PCR). Results: From 9 S. aureus resistant strains by disk diffusion 1 was sensitive by CIM, 7 CIM resistant strains were sensitive by disk diffusion. The 7 coagulase negative (CNS) sensitive strains by disk diffusion were resistant by CIM. By production of PBP2a, the results were discordant with the disk diffusion test in 20% and 34%with CIM. The genotype, reveals that, from 60 S.aureus strains 10(17%), and 7 S. coagulase negative strains 4 (57%) carry the mecA gene. From 10 S. aureus mecA positive strains, 5 carry the mecR1 gene and 7 carry the mecI gene. Of the 4 strains of S.coagulase negative mecA positive 2 carry the mecR1 and 2 carry the mecI gene. Conclusion: There is no association between genotype and phenotype in Staphylococcus spp. methicillin resistant strains, since, the resistance is due to many factors that the classical phenotypic test does not include.

Reactivity of penicillin-binding proteins with peptidoglycan-mimetic beta-lactams: what's wrong with these enzymes?

Beta-lactams exert their antibiotic action through their inhibition of bacterial DD-peptidases (penicillin-binding proteins). Bacteria, in general, carry several such enzymes localized on the outside of their cell membrane to catalyze the final step in cell wall (peptidoglycan) synthesis. They have been classified into two major groups, one of high molecular weight, the other of low. Members of the former group act as transpeptidases in vivo, and their inhibition by beta-lactams leads to cessation of bacterial growth. The latter group consists of DD-carboxypeptidases, and their inhibition by beta-lactams is generally not fatal to bacteria. We have previously shown that representatives of the former group are ineffective at catalyzing the hydrolysis/aminolysis of peptidoglycan-mimetic peptides in vitro [Anderson et al. (2003) Biochem. J. 373, 949-955]. The theme of these experiments is expanded in the present paper where we describe the synthesis of a series of beta-lactams (penicillins and cephalosporins) containing peptidoglycan-mimetic side chains and the kinetics of their inhibition of a panel of penicillin-binding proteins spanning the major classes (Escherichia coli PBP 2 and PBP 5, Streptococcus pneumoniae PBP 1b, PBP 2x and PBP 3, the Actinomadura R39 DD-peptidase, and the Streptomyces R61 DD-peptidase). The results of these experiments mirror and expand the previous results with peptides. Neither peptides nor beta-lactams with appropriate peptidoglycan-mimetic side chains react with the solubilized constructs of membrane-bound penicillin binding proteins (the first five enzymes above) at rates exceeding those of generic analogues. Such peptides and beta-lactams do react at greatly enhanced rates with certain soluble low molecular weight enzymes (R61 and R39 DD-peptidases). The former result is unexpected and interesting. Why do the majority of penicillin-binding proteins not recognize elements of local peptidoglycan structure? Possible answers are discussed. That this question needs to be asked casts fascinating shadows on current studies of penicillin-binding proteins for new drug design.