This once again favors the hypothesis that sigF is not strongly a

This once again favors the hypothesis that sigF is not strongly auto-regulated. Figure 4 Role of CC3252 on expression of CC2906, CC3255 and sigF genes . Results shown are from qRT-PCR performed with total RNA extracted from exponential growth phase cells under control conditions (no stress) or stressed with potassium dichromate (K2Cr2O7). We analyzed the parental strain NA1000 without expression plasmid pJS14, NA1000 with the empty plasmid pJS14 and NA1000 with pJS14 containing CC3252 gene (CC3252++). Values represent the fold increase

of CC2906, CC3255 and CC3253 (sigF) expression in the corresponding strain, exposed or not to the stress condition, compared with the parental strain NA1000 without pJS14 growing under control conditions. Results were normalized using gene CC0088 as the endogenous control, which was constitutively expressed check details in the

samples analyzed. Data are mean values of two independent experiments; bars represent the standard error. Statistical analysis is shown in Additional file 1: Table S4. A further attempt to investigate the role of nrsF as a possible negative regulator of σF function was carried out by click here trying to construct a null mutant strain in gene nrsF. However, it was not possible to construct a mutant strain by deleting nrsF in the parental strain (data not shown). On the other hand, nrsF could be deleted in the absence of a functional copy of sigF (data not shown), suggesting that high σF activity is apparently responsible for the failure of disrupting nrsF in cells with functional sigF. The putative protein encoded by nrsF is composed of six putative transmembrane segments separated by five short linkers (6 to 19 amino acid residues) and an N-terminal segment of 25 residues (Figure 5B). Alignment of the deduced amino acid sequence of CC3252 with its orthologs from other bacteria (Cupriavidus metallidurans,

Pseudomonas entomophila, Pseudomonas putida, Rhizobium leguminosarum, Maricaulis maris and Sinorhizobium meliloti) revealed two highly conserved cysteine residues (Figure 5A). The cysteine residues of the Caulobacter protein (positions 131 and 181) are probably directed into the periplasmic 4��8C space (Figure 5B), which favors their putative role in the signal transduction process leading to the liberation of σF from NrsF inhibition. Substitution of the conserved www.selleckchem.com/products/Temsirolimus.html cysteines by serine led to two single mutants (SG22, C131S; SG23, C181S) and a double mutant (SG24, C131S-C181S). Even under unstressed conditions, all σF-regulated genes analyzed in qRT-PCR experiments, including sigF and CC3252, were up-regulated in the single mutant strains when compared to the parental strain (Figure 5C). The substitution of both cysteines by serine in NrsF resulted in the highest expression levels of the genes analyzed (Figure 5C).

Comments are closed.