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Activity of glucose-fructose oxidoreductase in fresh and permeabilised cells of Zymomonas mobilis grown in different glucose concentrations

Atividade de glicose-frutose oxidorredutase em células íntegras e permeabilizadas de Zymomonas mobilis cultivadas em diferentes concentrações de glicose

Previously grown cells of the ethanologenic bacterium Zymomonas mobilis produce sorbitol and gluconic acid, in reactions catalysed by the periplasmic enzymes glucose-fructose oxidoreductase (GFOR) and glucono-delta-lactonase (GL). The GFOR/GL system activity, in cells to be used in this bioconversion, depends on growth conditions. In batch runs, with initial glucose concentrations (S0) from 42 to 230 g/L, the highest specific and total GFOR/GL activities were obtained with S0 = 153 g/L (12.6 U/g cells and 62 U/L). Higher S0 led to decreasing activities in fresh cells. With S0 = 209 g/L, the final specific activity was only 7.0 U/g. After disruption of cells, however, an activity over 15 U/g was revealed. Since growth inhibition with S0 over 153 g/L was observed in batch mode, fed-batch runs, equivalent to a batch of 230 g/L, were done. Although no growth inhibition occurred in fed-batch cultivation, enzyme activity remained low (5.2 U/g). A further fed-batch experiment, carried out under low pressure to remove ethanol from the medium, resulted in a specific activity of 9.8 U/g and a total activity of 68.7 U/L. These results indicate that the low GFOR/GL activities in Z. mobilis cells grown on higher S0 were due to changes in the cell wall, caused by high concentration of ethanol, that hindered the transport of the substrate to the intracellular enzymes in biconversion runs. This conclusion was confirmed by bioconversion runs with cells cultivated under different conditions.

Zymomonas mobilis; glucose-fructose oxidoreductase; glucose


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