The glycerol-3-phosphate transporter UgpB (spot ID 1229) was also induced under starvation, in BMS202 clinical trial agreement with similar observations in E. coli[32]. Interestingly, Brucella UgpB is cell-surface-located and plays a role as adhesin and invasin during infection Rabusertib price of epithelial cells [33]. Glycerol-3-phosphate is a metabolic intermediate of glycolysis and phospholipid biosynthesis, and Brucella may try to increase the take-up of such potential energy supplier to compensate

ATP deficiency. It remains to be investigated if UgpB has a double function in brucellae and whether a nutrient stress may promote subsequent invasion of host cells. The concentration of bacterioferritin (spot ID 2176), the major actor in iron homeostasis, was also increased under starvation conditions with low levels of iron. It has been described previously that the bacterioferritin-related iron pool induces membrane proteins to adapt to low iron concentrations, confirming the central role of bacterioferritin

in the iron storage of Brucella[34]. During starvation, two enzymes involved in leucine and glutamate biosynthesis, 3-isopropylmalate-dehydrogenase (spot ID 1915) and carbamoylphosphate synthase (spot ID 221), respectively, were repressed, indicating that the bacteria reduced their Selleck BAY 11-7082 metabolic activity. In contrast, concentration of the glycine cleavage system P protein (spot ID 278) increased. This protein is part of the glycine decarboxylase multienzyme complex, also annotated as glycine cleavage system, and functions as a glycine dehydrogenase. In a signature-tagged mutagenesis screen investigating long-term survival of B. abortus in mice, the P protein was identified as a factor participating

in chronic PTK6 persistence of the pathogen [35]. In M. tuberculosis, the activity of glycine dehydrogenase has been found to increase 10-fold upon entry into a state of nonreplicating persistence in vitro[6]. Another protein of this system, GcvT, has been described thereafter as being essential in intramacrophagic survival of B. suis[3]. Since this enzyme catalyzes the step resulting in release of NH3, activity of the glycine decarboxylase multienzyme complex may allow starving bacteria to recycle ammonium residues from glycine metabolism for minimal biosynthetic activities required under these conditions. In addition, concentrations of several amino acid transporters increased (spot ID 1219, 1293, and 1549), which is in agreement with other studies describing their positive regulation by the stringent response allowing bacteria optimal adaptation to starvation (reviewed in [36]). In the group of factors linked to protein metabolism, two ribosomal proteins (spot ID 1783 and 1980) were starvation-induced. This seems to be contradictory to the obvious shut-down of cellular metabolism.