The role of nitrogenase in a cyanide-degrading Klebsiella oxytoca strain.

Abstract

It is well known that the major function of nitrogenase is to fix atmospheric nitrogen. However, cyanide can also serve as a subtrate for nitrogenase and can be reduced to CH4 and NH4+. A cyanide-degrading Klebsiella oxytoca strain was isolated from cyanide contaminated water. This isolate was also found to have a nitrogen-fixation capability. Nitrogenase activities in this organism could be induced by KCN. However, there was no significant difference of the induction effect between 1 mM KCN and 5 mM KCN. It was found that the cyanide-degrading ability of this isolate could be inhibited by multicopy hybrid pGR112 nif-containing plasmids. Comparing the wild type K. oxytoca strain with the pGR112 plasmid transformed strain, a typical diauxic growth of the wild type strain was observed in a medium containing NH4Cl and KCN. Although the nif plasmid transformed strain also exhibited diauxic growth in the same medium, a much longer second lag phase was noted. In addition, methane, the nitrogenase reduction end product of cyanide, could be detected on cyanide-containing growth cultures. Ammonium chloride, a repressor of nitrogenase gene expression, was consumed prior to KCN in both strains. Again, the degradation of KCN in the pGR112 transformed strain occurred only under loose control of the nitrogenase gene. These findings strongly suggest that nitrogenase may be the sole cyanide-degrading enzyme in this organism.