aureus virulence in silkworms Protein A contributes to the virul

aureus virulence in silkworms. Protein A contributes to the virulence of S. aureus by interacting with immunoglobulin in mammalian blood (Palmqvist et al., 2002). The lack of the requirement for spa in S. aureus infection of silkworms is presumably due to the absence of immunoglobulin in invertebrates, including silkworms. We demonstrated that cell-wall-anchored proteins, ClfB, FnbB and MK2206 SdrC, contributed

to the virulence of S. aureus in silkworms. To our knowledge, this is the first report that cell-wall-anchored proteins contribute to the virulence of S. aureus in an invertebrate model animal. ClfB binds cytokeratins of mammalian epithelial cells and the interaction is required for S. aureus colonization onto nasal epithelial cells (Wertheim et al., 2008); FnbB binds mammalian fibronectin and contributes to the virulence of S. aureus (Palmqvist et al., 2005); and SdrC is required for adherence of S. aureus to mammalian epithelial cells (Barbu et al., 2008; Corrigan et al., 2009). Therefore, ClfB, FnbB and SdrC are presumably required PF-01367338 solubility dmso for adherence of S. aureus to silkworm tissues

by binding silkworm proteins that are homologous to the mammalian target proteins. Invertebrate animal models of S. aureus infection include C. elegans, D. melanogaster and Manduca sexta, in addition to silkworms (Sifri et al., 2003; Needham et al., 2004; Fleming et al., 2006). In the C. elegans model, bacteria were eaten by worms and the number of surviving worms was counted (Sifri et al., 2003). In the D. melanogaster model, bacteria were injected into adult flies by injuring animals with tungsten needles that were dipped in a solution containing bacteria, and the number of surviving flies was counted (Needham et al., 2004). In the M. sexta model, bacteria were injected into larvae by using microsyringes (Fleming

et al., 2006). In the C. elegans model, the agr locus, saeRS and hla genes of S. aureus are required to kill worms, although srtA is not (Table 3) (Sifri et al., 2003; Bae et al., 2004). In the D. melanogaster model, Ketotifen the agr locus, saeRS and arlRS of S. aureus were not required for killing flies (Table 3) (Needham et al., 2004). In the M. sexta model, the agr locus of S. aureus is involved in killing larvae (Table 3) (Fleming et al., 2006). Our present study revealed that agr, saeRS, arlRS and srtA of S. aureus were required for killing silkworms, whereas hla was not required. The different results between these animal models may be due to different sensitivities of animals against exotoxins, different adhesive characteristics of cell surfaces to bacterial cells, and different experimental conditions, such as temperatures and infection routes. The findings of the present study revealed that genes encoding hemolysins of S. aureus are not required for killing silkworms, whereas some genes encoding cell-wall proteins and regulatory proteins are required.

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