DL-Tetrahydrofolate (THF) and ATP were necessary for the anaerobic 0-demethylation of phenylmethylethers in cell extracts of the type strain (ATCC 29683) of the homoacetogen Acetobacterium woodii. The reactants for this enzymatic activity have not been previously demonstrated in any system, nor has the mediating enzyme been studied. An assay using reaction mixtures containing 1 mM THF, 2 mM ATP, and 2 mM hydroferulate (i.e., 4-hydroxy,3-methoxyphenylpropionate) was developed and was performed under stringent anaerobic conditions. Pyridine nucleotides and several other possible cofactors were tested but had no effect on the activity. After centrifugation of disrupted cells at 27,000 x g, the activity was found primarily in the supernatant, which had a specific activity of 14.2 + 0.5 nmol/min/mg of protein. At saturating levels of each of the other two substrates, apparent Km values for the variable substrate were 0.65 mM hydroferulate, 0.27 mM ATP, and 0.17 mM THF. Activity was significantly decreased when extract was preincubated at 60°C and was completely lost after preincubation in air for 30 min. Thus, the soluble anaerobic 0-demethylating enzyme system of A. woodii is oxygen sensitive. The THF-and ATP-dependent activity measurable in the soluble fraction of cell extracts constituted about 34% of the activity seen with intact cells.
A novel strain of gram-negative anaerobic rods which utilized 0-methyl substituents of monoaromatic acids as a sole organic source of carbon was isolated from municipal sewage sludge. Energy for growth seemed to be generated by an acetate formation pathway. The growth yield in defined medium was 7.9 g (dry weight) of cells per mol of ferulate utilized. This isolate and other O-demethylating anaerobes may play a role in the turnover of acetate and the metabolism of highly methoxylated lignaceous materials in anaerobic environments.
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