Figure 2 Swimming motility by G3 is independent of AHL signalling

Figure 2 Swimming motility by G3 is independent of AHL selleck inhibitor signalling. One microlitre of overnight cultures of the wild type G3 (A), the control G3/pME6000

(B) and G3/pME6863-aiiA (C) were inoculated onto swim agar plates and incubated at 28°C for 16 h. Lactonase expression in S. plymuthica G3 reduces antifungal activity in vitro Strain G3 exhibited inhibitory effects against several phytopathogenic fungal isolates in vitro and in vivo (data not shown). To determine the effect of quorum quenching by lactonase on antifungal activity, dual cultures were carried out, on single PDA plates, of the strain G3, G3/pME6863-aiiA or G3/pME6000 with C. parasitica, p38 MAP Kinase pathway the cause of chestnut blight. After incubation for 4 days at 25°C, the radius of the inhibition zones was measured. Although no large differences

were observed between the wild type G3 and the control strain G3/pME6000, the radius of inhibition zones produced by G3/pME6863-aiiA was significantly decreased compared with the control G3/pME6000 and the wild type G3 at P = 0.01 for C. parasitica (Table 3.). The data showed that antifungal activity by G3 is partially dependent on AHL signaling via regulation of various exoenzymes and secondary metabolites. Table 3 Effect of quorum quenching on antifungal activity in vitr o Phytopathogenic fungus Inhibition zone (mm)*   G3 (wt) G3/pME6863- www.selleckchem.com/products/Vorinostat-saha.html aiiA G3/pME6000 Cryphonectria parasitica a 8.25 ± 0.42 (A) 5.91 ± 0.20 (B) 8.33 ± 0.51 (A) * Radius of inhibition zone on PDA plates in dual culture for 4 days, Data represents mean values ± SD with six replicates. a Different letters in

the same line indicate significant differences at P < 0.01 Abiotic surface adhesion and biofilm formation in S. plymuthica G3 are affected by lactonase expression Many bacteria rely on QS systems to govern various aspects of biofilm development, including adhesion, motility, maturation, and dispersion [10, 37]. Using microtiter plate assays, we evaluated the impact of quorum quenching by aiiA on adhesion to abiotic surfaces in G3. Figure 3A illustrates by OD600, there are no significant difference in bacterial growth rate between the wild type G3, G3/pME6000 and G3/pME6863-aiiA, but the strain G3/pME6863-aiiA showed a significant reduction in adhesion, compared with heptaminol the vector control strain G3/pME6000 and the wild type G3 (Figure 3B). Figure 3 Effect of aiiA expression on abiotic surface adhesion by S. plymuthica G3. A: OD600 of G3 bacterial cultures in the presence and absence of the aiiA lactonase gene. B: Absorbance of crystal violet at 570 nm from stained cells bounds to polystyrene microtitre plate as a representation of adhesion. Experiments were done in triplicate. Furthermore, 48 hour flow cell cultures of GFP-tagged G3/pME6863-aiiA and G3/pME6000 were observed and quantified for biofilm formation using CLSM during two independent experiments.

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