TatB (specifies a WT copy of tatB), and pRB.TAT. Panel C: Growth of O35E is compared to that of its tatC isogenic mutant strain, O35E.TC, carrying the plasmid pWW115 and pRB.TatC (contains a WT copy of tatC). Growth of the bro-2 isogenic mutant strain O35E.Bro is also shown. The results are shown as a composite image representative

of individual experiments that were performed in duplicate on at least 3 separate occasions. The effect of tat mutations on the β-lactamase activity of M. catarrhalis was quantitatively measured using the chromogenic β-lactamase substrate nitrocefin. These assays were performed using suspensions of freshly plate-grown bacteria placed into the wells of a 48-well tissue culture plate. A solution containing nitrocefin was added ATM Kinase Inhibitor mw to these suspensions and the change of color from yellow to red (indicative of cleavage of the β-lactam ring) was monitored by measuring the absorbance of well contents at a wavelength of 486 nm. Substantially less β-lactamase activity was observed for the tatA, tatB and tatC mutants compared to the WT strain O35E (Figure 6). Complementation of the tatA and tatB mutants with plasmids containing only the WT copies of the inactivated genes did not restore β-lactamase activity, as expected based on the results of the experiments

depicted in Figures 3 and 5. The plasmid pRB.TAT, which specifies the entire tatABC locus, restored the ability of the mutants O35E.TA (Figure 6A) EPZ-6438 cost and O35E.TB (Figure 6B) to hydrolyze nitrocefin. The plasmid pRB.TatC was sufficient to rescue β-lactamase activity in the tatC mutant strain O35E.TC to near WT levels (Figure 6C). The tatC mutant of strain O12E was tested in this manner and the results were consistent with those obtained with O35E.TC (data not shown). Cobimetinib The control strain, O35E.Bro, was impaired in its ability to hydrolyze nitrocefin at levels comparable to those of the tatA, tatB and tatC mutants (Figure 6A, B and C). Taken together, these results suggest that the M. catarrhalis tatABC locus is necessary for secretion of the β-lactamase BRO-2 into the periplasm where the enzyme can protect the peptidoglycan

cell wall from the antimicrobial activity of β-lactam antibiotics. Figure 6 Quantitative measurement of the β-lactamase activity produced by the M. catarrhalis WT isolate O35E and tat mutant strains. The β-lactamase activity of strains was measured using the chromogenic compound nitrocefin. Bacterial suspensions were mixed with a 250 μg/mL nitrocefin solution and the absorbance at 486 nm (A486) was immediately measured and recorded as time “0” (open bars). The A486 of the AR-13324 samples was measured again after a 30-min incubation at room temperature (black bars). Panel A: The β-lactamase activity of O35E is compared to that of the tatA mutant strain, O35E.TA, carrying the plasmid pWW115 (control), pRB.TatA (specifies a WT copy of tatA), and pRB.TAT (harbors the entire tatABC locus).