pylori [36] In the current study, the

three mutant VacA

pylori [36]. In the current study, the

three mutant VacA proteins that exhibited the most striking defects in secretion (Δ559-579, Δ580-607, Δ608-628) each contained deletions that are localized near the carboxy-terminus of the β-helix. Interestingly, a study of Bordetella pertussis BrkA revealed that a β-helical region near the carboxy-terminus of the passenger domain is required for folding of this protein [44]. The authors proposed that this domain acts as an intramolecular chaperone to promote folding of the passenger domain concurrent with or following translocation through the outer membrane. Similarly, selleck inhibitor studies of B. pertussis pertactin indicate that the carboxy-terminal β-helical region

of this protein exhibits enhanced stability and can fold PRIMA-1MET price as a stable core structure [5, 45]. We speculate that VacA amino acids 559-628 have a similar functional role in promoting protein folding and secretion. An important finding in the current study is that, within the VacA β-helix, there are regions of plasticity that tolerate alterations without detrimental effects on protein secretion or toxin activity. VacA Δ484-504, Δ511-536, and Δ517-544 mutant proteins each retained vacuolating activity similar to that of wild-type VacA, which indicates that the corresponding coils are dispensable for vacuolating toxin activity. The retention of vacuolating activity despite the deletion of entire coils of the β-helix correlates well with results from a previous study, which reported that inactivating point mutations within the portion of vacA encoding the p55 domain could not be identified [26].

One of the VacA mutant proteins analyzed in the current study (Δ433-461) exhibited detectable vacuolating toxin activity on HeLa Rutecarpine cells, but its activity on HeLa cells was reduced compared to that of wild-type VacA, and it lacked detectable activity on RK13 cells and AZ521 cells. These data suggest that residues within this VacA region (amino acids 433-461) have an important role in VacA activity. Further studies may lead to the identification of specific amino acids within this region that STAT inhibitor mediate interactions between VacA and host cells. Similar to most previous studies, the current study assessed the effects of VacA mutations on the ability of VacA to cause cell vacuolation. Future investigations may provide new insights into structural properties of VacA that are required for other actions of this multifunctional toxin. Conclusions VacA is a unique toxin that is considered to be an important determinant of H. pylori virulence, and therefore, it is important to have an in-depth understanding of VacA structure and function. The VacA p55 structure is predominantly a right-handed parallel β-helix, which is a characteristic of autotransporter passenger domains.

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