Hence, it is possible that the ComS peptide may also function int

Hence, it is possible that the ComS peptide may also function intracellularly without its export and subsequent import into the cell. We have also taken into consideration that conditions tested in complex medium may not be optimal for the expression

of the XIP exporter, which can likely result in the accumulation of ComS inside the cell, making it vulnerable to intracellular cleavage. Our expression analysis combined with LC-MS/MS in CDM demonstrates a negative-regulatory role for the ComDE Ipatasertib concentration system in XIP production. Kreth et al. (2007) reported that ComDE repressed comC expression prior to CSP stimulation. It is possible that ComDE may prevent premature expression of comS, thereby delaying competence induction in CDM to the latter stages of growth. As MK-8669 supplier observed by Desai et al. (2012), competence in CDM is first observed in mid-logarithmic cells of S. mutans and continues well into the stationary phase. We further observe that the amount of XIP was significantly reduced in ∆SMcomX, suggesting a ComX-mediated positive feedback mechanism for XIP synthesis. Putative ComX binding sites were located within the comR gene, upstream of comS, suggesting that ComX may directly

regulate comS expression (Fig. 6a). This positive autoregulation of XIP production may contribute to the persistence of the competent state in CDM. Based on previous works and our findings presented here, we Sinomenine propose a growth condition–dependent model for genetic competence in S. mutans (Fig. 6b). We thank Kirsten Krastel for technical assistance. We are thankful to Dr. Donald Morrison for his review of our manuscript and helpful suggestions provided along with Dr. Lauren Mashburn-Warren and Dr. Mike Federle. D.G.C. is a recipient of the NIH grant R01DE013230-03 and CIHR-MT15431. “
“Bacillus sp. strain CS93, which was previously isolated from Pozol, was previously shown to produce iturin A, bacilysin and chlorotetaine. To investigate the biosynthetic

mechanism of chlorotetaine production, the bac genes were amplified from genomic DNA of Bacillus sp. CS93 by PCR and sequenced. The genes bacABCDE were determined, but no gene that might code for a halogenating enzyme was detected either within the gene cluster or in the flanking sequences. Following further analysis of culture supernatants that were active against bacteria by liquid chromatography-MS, it was not possible to detect bacilysin/chlorotetaine. However, in methanolic fractions containing antibacterial activity, molecular ions characteristic of surfactins and fengycin were detectable by electrospray MS. Using primers complementary for conserved regions of nonribosomal peptide synthase, it was possible to amplify gene fragments that had a high degree of homology with known surfactin and fengycin biosynthetic genes.

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