The results of the Oxyblot assay showed that the ΔmglA mutant contained significantly more oxidized proteins
than LVS under aerobic conditions. Reactive oxygen species are generated as a byproduct of the normal metabolism of a growing organism and PFT�� mw there is, therefore, a continuous need to neutralize them to avoid oxidative damage of macromolecules in the cell. In view of this, the high level of oxidized proteins in ΔmglA strongly suggests that MglA has a central role for the normal oxidative stress response and that its absence renders F. tularensis severely impaired to handle reactive oxygen species leading to specific protein damage which hampers the bacterial growth. In support of this, previously published data on the F. learn more novicida mglA mutant revealed that key enzymes in the glutaredoxin systems, such as gluthathione synthetase, glutaredoxine, and thioredoxine, all of which have critical roles to neutralize reactive oxygen species [29], were selleck screening library greatly repressed [9, 10]. A rational adaptation to the increased oxidative stress encountered by ΔmglA would be to decrease the iron-driven Fenton reaction, which otherwise will result in the generation of highly reactive hydroxyl anions and radicals [17]. The most effective way to do this would be to limit the intracellular iron pool and upregulate the expression of catalase. Such an adaptation
to oxidative stress has been noted in for example E. coli [18]. Our results support such
a scenario also for F. tularensis Methocarbamol since catalase was upregulated, thereby enhancing the capability of the bacterium to sustain an oxidative stress, and the expression of the fsl operon and feoB was suppressed in ΔmglA under aerobic conditions. Moreover, ΔmglA regulated iron-uptake genes similarly to LVS under microaerobic conditions and under severe iron-deprivation. This indicates that the marked downregulation of iron uptake genes observed under aerobic conditions does not relate to any inherent defects with regard to iron uptake, but instead is a compensatory mechanism needed to avoid the deleterious effects of the Fenton reaction. An alternative explanation to the suppressed expression of the fsl operon and feoB in ΔmglA could be high availability of iron in the medium. However, we found no correlation between iron content and the fsl regulation, which further supports the hypothesis that oxidative stress was the primary reason for the dysregulation of the fsl operon and feoB in ΔmglA under aerobic conditions. We hypothesized that the growth of ΔmglA in the microaerobic milieu would reduce the oxidative stress. Indeed, the levels of oxidized proteins in the ΔmglA mutant were normalized and similar to those found in LVS and, moreover, the growth of the mutant was similar to LVS.