012 μmol/min/mg [40]. It should also be noted that the histidine phosphatase superfamily typically contains the characteristic motif ‘RHG’ at the N-terminal region. However, the motif present in Rv2135c is ‘RHA’ as found in the yet uncharacterized phosphoglycerate domain containing protein of C. parvum (GAN CAD98474). The replacement of glycine with alanine, another non-polar amino acid with a small side chain, may occur without any effect on the specificity of the enzymes in this family. Moreover, Rv2135c contains other residues reported to be important in
the phosphatase activities of other members of the superfamily. These include Arg57, Glu82, and a fully conserved His153 at the C-terminal region [3, 9, 36]. Thus, we believe that Rv2135c AZD1390 cost performs an acid phosphatase function Akt inhibitor in its native environment. The substrate specific to Rv2135c is unknown. Its sequence appeared to have little similarity to other previously annotated histidine phosphatases of M. tuberculosis[17], although the annotations of most of these phosphatases are still computational. Therefore there is no information suggesting the primary substrate of the enzyme. There are few experimentally characterized phosphatases in M. tuberculosis. These include Rv3214 and Rv2419c, which are histidine phosphatases [3,
17], PtpA and PtpB which are tyrosine protein phosphatases [41, 42], and PstP, a serine/threonine protein phosphatases [43]. The specific substrates of these phosphatases have not been identified yet, with the exception of Rv2419c, a glucosyl-3-phosphoglycerate phosphatase [17]. There are several known functions of histidine acid phosphatases, including extracellular metabolism, scavenging and regulatory functions. Rv2135c was identified as being associated with membrane protein
this website fractions [20, 44]. M. tuberculosis encounters a phosphate deficient acidic environment in an infected macrophage, and has been shown to depend on the acquisition of phosphate groups from the host environment for survival [29]. It is therefore intriguing to further study whether Rv2135c plays some roles in the intramacrophage environment, where it has been shown to be expressed [45]. Rv2135c and Rv2136c have been predicted to be in the same operon (http://genome.tbdb.org/annotation/genome/tbdb/). Rv2136c is the only mycobacterial gene with the catalytic motif of undecaprenyl pyrophosphate phosphatase. In bacteria, the enzyme hydrolyzes undecaprenyl pyrophosphate to produce undecaprenyl phosphate needed to translocate various cell wall intermediates from the cytosol across the cytoplasmic membrane for polymerization [46, 47]. selleck compound Despite the apparent essentiality of this function, undecaprenyl pyrophosphatases of many bacteria are known to be non-essential for their growth [48, 49]. Rv2136c has also been shown to be non-essential for the survival of M. tuberculosis[50]. In some bacteria such as E.
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