Sulfate-reducing bacteria are characterized by a high number of hydrogenases, which have been proposed to contribute to the overall energy metabolism of the cell, but exactly in what role is not clear. Desulfovibrio spp. can produce or consume H 2 when growing on organic or inorganic substrates in the presence or absence of sulfate. Because of the presence of only two hydrogenases encoded in its genome, the periplasmic HynAB and cytoplasmic Ech hydrogenases, Desulfovibrio gigas is an excellent model organism for investigation of the specific function of each of these enzymes during growth. In this study, we analyzed the physiological response to the deletion of the genes that encode the two hydrogenases in D. gigas, through the generation of ⌬echBC and ⌬hynAB single mutant strains. These strains were analyzed for the ability to grow on different substrates, such as lactate, pyruvate, and hydrogen, under respiratory and fermentative conditions. Furthermore, the expression of both hydrogenase genes in the three strains studied was assessed through quantitative reverse transcription-PCR. The results demonstrate that neither hydrogenase is essential for growth on lactate-sulfate, indicating that hydrogen cycling is not indispensable. In addition, the periplasmic HynAB enzyme has a bifunctional activity and is required for growth on H 2 or by fermentation of pyruvate. Therefore, this enzyme seems to play a dominant role in D. gigas hydrogen metabolism.
Hydrogenases are key enzymes in the hydrogen metabolism of Desulfovibrio spp. that catalyze the reversible oxidation of molecular hydrogen into protons and electrons (1). However, their role during sulfate respiration has not been clearly established. Odom and Peck proposed a hydrogen cycling model to explain energy conservation during growth on lactate and sulfate by Desulfovibrio spp., which belong to the deltaproteobacteria subgroup of the sulfate-reducing bacteria (SRB) (2). The model predicts that protons and electrons produced in the oxidation of lactate are used for the production of molecular hydrogen by a cytoplasmic hydrogenase. This hydrogen then diffuses across the membrane to the periplasm, where it is reoxidized by a periplasmic hydrogenase. Electrons are transferred back to the cytoplasm for sulfate reduction, thus creating a proton gradient across the membrane that leads to ATP formation. In this model, the presence of at least two hydrogenases on opposite sides of the membrane is a requirement for growth. In contrast, other studies suggested that the physiological role of these enzymes was to regulate the redox potential of the cell, controlling the flow of protons and electrons and generating a proton motive force (3). More recent models, proposed for Desulfovibrio vulgaris, suggested dual pathways for electron transfer from lactate to sulfate, one involving the cycling of H 2 and the other a route involving a membrane-associated electron transfer chain (4, 5). Several membrane complexes have been identified in SRB that could be involved in this proce...
