epidermidis stain harboring PQG56 (spx antisense knock-down plasm

epidermidis stain harboring PQG56 (spx antisense knock-down plasmid) is increased substantially, in accordance with the phenotype in the homologous spx mutant strain of S. aureus (Pamp et al., 2006). This observation further supports that spx is an important regulator mediating the biofilm formation of S. epidermidis. Biofilm formation by S. epidermidis

is generally considered as a two-step process, including primary attachment and biofilm accumulation. To investigate selleck chemical which step is affected by Spx, we first compared the attachment ability of the Spx-overexpressing strain (harboring pQG55) and the vector control strain (harboring pQG53). In primary attachment assays, the Spx-overexpressing strain showed decreased attachment ability (about 34-fold) to polystyrene compared with the WT strain, whereas the strains carrying either pQG53 or pQG54 showed no difference in primary attachment (Fig. 3a and b). To investigate whether the transcription of atlE was affected Belnacasan by Spx, quantitative RT-PCR was performed. The result indicates that the transcriptional level of atlE in the Spx-overexpressing strain carrying pQG55 shows no difference compared with the other three strains (Fig. 3c). This indicates that Spx does not affect the attachment ability by regulating

atlE. We then compared the primary attachment on 96-well polyethylene plates between WT and ica-negative strains isolated from our previous work (Li et al., 2005), and no significant difference was found (data not shown). PIA is a key factor in the biofilm accumulation of S. epidermidis (Rupp et al., 1999). To investigate whether the production of PIA was affected by Spx, immuno-dot blot PDK4 assays were performed. The Spx-overexpressing strain was found to produce significantly less PIA compared with the vector control strain (Fig. 4a). The transcription of the icaADBC operon and its repressor icaR among different strains was further examined by quantitative RT-PCR. Decreased

icaADBC, but comparable icaR transcriptional levels were found in the Spx-overexpressing strain compared with the vector control strain (Fig. 4b and c). This result indicates that Spx affects PIA production by regulating the transcription of icaADBC in an icaR-independent manner. In B. subtilis and S. aureus, Spx plays an important role in the oxidative-stress adaptation. The B. subtilis and S. aureus spx mutant strains were hypersensitive to diamide, a thiol-specific oxidant (Nakano et al., 2003a; Pamp et al., 2006). To study whether the overexpression of Spx affects S. epidermidis in the adaptation to diamide, the diamide sensitivity of the Spx-overexpressing strain (harboring pQG55) and the control strain (harboring pQG53) was compared using disk diffusion tests.

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