SCREENING AND SELECTION OF WILD STRAINS FOR L-ARABINOSE ISOMERASE PRODUCTION

MANZO, RICARDO; SIMONETTA, ARTURO; RUBIOLO, AMELIA C; MAMMARELLA, ENRIQUE J

BRAZILIAN JOURNAL OF CHEMICAL ENGINEERING

BRAZILIAN SOC CHEMICAL ENG

Lugar: BRASIL; Año: 2013 vol. 30 p. 711 - 720

0104-6632

The majority of L-arabinose isomerases have been isolated by recombinant techniques, but this methodology implies a reduced technological application. For this reason, 29 bacterial strains, some of them previously characterized as L-arabinose isomerase producers, were assayed as L-arabinose fermenting strains by employing conveniently designed culture media with 0.5% (w/v) L-arabinose as main carbon 1 source. From all evaluated bacterial strains, Enterococcus faecium DBFIQ ID: E36, Enterococcus faecium DBFIQ ID: ETW4 and Pediococcus acidilactici ATCC ID: 8042 were, in this order, the best L-arabinose fermenting strains. Afterwards, to assay L-arabinose metabolization and L-arabinose isomerase activity, cell-free extract and saline precipitated cell-free extract of the three bacterial cultures were obtained and the production of ketoses was determined by the cysteine carbazole sulfuric acid method. Results showed that the greater the L-arabinose metabolization ability, the higher the enzymatic activity achieved, so Enterococcus faecium DBFIQ ID: E36 was selected to continue with production, purification and characterization studies. This work thus describes a simple microbiological method for the selection of L arabinose fermenting bacteria for the potential production of the enzyme L-arabinose isomerase.