In contrast to VP1680, the VopA TTSS2 effector has been found to inhibit MAPK in macrophages by acetylating the upstream MAPK Kinase (MKK) [18, 30]. It is important to note that the VopA studies were selleck inhibitor performed with transfected eukaryotic cells that expressed VopA heterologously, whereas the current study assessed MAPK check details activation by intact V. parahaemolyticus.
From our studies during co-incubation of V. parahaemolyticus with Caco-2 cells it appears that the MAPK activation of VP1680 is dominant over the inhibitory effect of VopA. V. parahaemolyticus may co-ordinately regulate both TTSS to achieve appropriate control of host responses. V. parahaemolyticus induced IL-8 secretion in an Volasertib order active manner as a result of delivery of the TTSS effector proteins into host cells (Figure 5). It appears that there may be a balance between TTSS1 and TTSS2 of V. parahaemolyticus where TTSS1 is involved in the activation of IL-8 production by the host while TTSS2 is involved in its inhibition. This correlates with the opposing functions of the TTSS1 effector
VP1680 and the TTSS2 effector VopA in activating and inhibiting MAPK phosphorylation. Interestingly, the TTSS1 effector VP1680 mutant (Δvp1680) induced intermediate amounts of IL-8, suggesting an involvement of this protein in stimulating production of this chemokine, but not an absolute requirement (Figure 5). Similarly the inhibitory studies revealed that V. parahaemolyticus induces secretion of IL-8 partly via
modulation of the ERK signalling pathway (Figure 6). The complex effect of both TTSS of V. parahaemolyticus on the host immune defence machinery illustrates the powerful tools the bacteria possess to gain maximum advantage from the host environment. Conclusions A better understanding of the virulence mechanisms of V. parahaemolyticus is imperative for better diagnosis, treatment and prevention of gastrointestinal infections. The findings presented here provide new insights into the roles of TTSS1 and TTSS2 in modulating epithelial cell responses to infection. V. parahaemolyticus induced JNK, ERK Protein tyrosine phosphatase and p38 activation in human epithelial cells. TTSS1, and the TTSS1 effector VP1680, were of key importance for sabotaging normal MAPK cellular processes and disrupting host responses to infection. MAPK activation was associated with the cytotoxic effects exerted by the bacterium and with the induction of IL-8 secretion. The diverse roles of MAPK signalling during infection with V. parahaemolyticus indicate it is a significant mechanism to promote virulence. Methods Cells and reagents V. parahaemolyticus RIMD2210633, O3:K6 serotype (wild type, WT) [12] was used for the construction of deletion mutants as well as to perform all experiments.