In contrast, SecA (spot ID 313), participating in protein

In contrast, SecA (spot ID 313), participating in protein translocation/secretion, was found in lower concentrations in starved Brucella, indicating an additional strategy to reduce metabolic activity and energy consumption. In analogy to the observed repression of amino acid biosynthesis, energy-consuming de novo DNA and RNA biosynthesis was also reduced. RNA degradation increased,

indicating a higher turnover than under control conditions and enabling bacteria to rapidly recycle the corresponding molecules. Increased degradation was also noticed for fatty acids, leading to the speculation that brucellae might use own fatty acids for minimum energy supply. Indeed, the induction of a putative long-chain Quisinostat clinical trial acyl-CoA thioester hydrolase (spot ID 1881) has been previously observed under anaerobic denitrification, suggesting a switch to β-oxidation for energy supply under anaerobic stress conditions [14]. In the group of energy metabolism-related proteins, one single subunit of the ATP synthase (spot ID 1019) was identified as being induced under starvation conditions as compared to early stationary phase in rich medium, indicating that Brucella attempts to counteract obvious ATP limitation. As membrane-associated proteins are not systematically

separated in 2D gel electrophoresis, the identification of only one ATP synthase subunit was conceivable. Thioredoxin (spot ID 1435) participates in NADPH-dependent formation of disulfide bonds in target proteins [37], hence consuming reduction equivalents are no longer available for electron transport and ATP find more synthesis. The decrease in thioredoxin under starvation stress is in agreement with the observed reduction

in amino acid (and therefore protein) biosynthesis, resulting in energy saving. A single protein involved in oxido-reduction, click here alkylhydroperoxide reductase C (spot ID 1975), has been identified as being down-regulated Montelukast Sodium under these extreme starvation conditions. In B. subtilis, AhpC was postulated to be responsible for the detoxification of endogenous organic hydroperoxides arising from unsaturated fatty acids and from nucleic acids during growth under oxidative stress [38]. In Brucella abortus, AhpC is the primary detoxifier of endogenous H2O2 generated by aerobic metabolism [39]. Down-regulation of this enzyme in brucellae was therefore in accordance with a reduced oxidative bacterial metabolism during long periods of starvation with absence of noticeable growth. Spots 2172, 2207, and 1455 (see Additional file 1) were identified as being significantly regulated (p ≤0.05), but the low concentrations of these proteins in the samples did not allow their identification. Conclusions The aim of this work was to gain a deeper insight into the regulative processes of B.

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