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Appl. Environ. Microbiol., 02 1995, 526-530, Vol 61, No. 2
BT Hopkins, MJ McInerney and V Warikoo
An anaerobic, motile, gram-negative, rod-shaped, syntrophic, benzoate-
degrading bacterium, strain SB, was isolated in pure culture with crotonate
as the energy source. Benzoate was degraded only in association with an
H2-using bacterium. The kinetics of benzoate degradation by cell
suspensions of strain SB in coculture with Desulfovibrio strain G-11 was
studied by using progress curve analysis. The coculture degraded benzoate
to a threshold concentration of 214 nM to 6.5 microM, with no further
benzoate degradation observed even after extended incubation times. The
value of the threshold depended on the amount of benzoate added and,
consequently, the amount of acetate produced. The addition of sodium
acetate, but not that of sodium chloride, affected the threshold value;
higher acetate concentrations resulted in higher threshold values for
benzoate. When a cell suspension that had reached a threshold benzoate
concentration was reamended with benzoate, benzoate was used without a lag.
The hydrogen partial pressure was very low and formate was not detected in
cell suspensions that had degraded benzoate to a threshold value. The Gibbs
free energy change calculations showed that the degradation of benzoate was
favorable when the threshold was reached. These studies showed that the
threshold for benzoate degradation was not caused by nutritional
limitations, the loss of metabolic activity, or inhibition by hydrogen or
formate. The data are consistent with a thermodynamic explanation for the
existence of a threshold, but a kinetic explanation based on acetate
inhibition may also account for the existence of a threshold.
Copyright © 1995, American Society for Microbiology
Evidence for anaerobic syntrophic benzoate degradation threshold and isolation of the syntrophic benzoate degrader
Department of Botany and Microbiology, University of Oklahoma, Norman 73019-0245, USA.
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