flaA1 and wbpB are conserved genes with unknown biological function in Helicobacter pylori. Since both genes are predicted to be involved in lipopolysaccharide (LPS) biosynthesis, flagellum assembly, or protein glycosylation, they could play an important role in the pathogenesis of H. pylori. To determine their biological role, both genes were disrupted in strain NCTC 11637. Both mutants exhibited altered LPS, with loss of most O-antigen and core modification, and increased sensitivity to sodium dodecyl sulfate compared to wild-type bacteria. These defects could be complemented in a gene-specific manner. Also, flaA1 could complement these defects in the wbpB mutant, suggesting a potential redundancy of the reductase activity encoded by both genes. Both mutants were nonmotile, although the wbpB mutant still produced flagella. The defect in the flagellum functionality of this mutant was not due to a defect in flagellin glycosylation since flagellins from wild-type strain NCTC 11637 were shown not to be glycosylated. The flaA1 mutant produced flagellins but no flagellum. Overall, the similar phenotypes observed for both mutants and the complementation of the wbpB mutant by flaA1 suggest that both genes belong to the same biosynthesis pathway. The data also suggest that flaA1 and wbpB are at the interface between several pathways that govern the expression of different virulence factors. We propose that FlaA1 and WbpB synthesize sugar derivatives dedicated to the glycosylation of proteins which are involved in LPS and flagellum production and that glycosylation regulates the activity of these proteins.Helicobacter pylori is a spiral-shaped gram-negative microaerophilic bacterium that was first isolated from the human stomach in 1984 (42). It is estimated that 70% of the worldwide population is infected by this bacterium. Most infections are asymptomatic, but they can also lead to gastric ulcers and cancers (26,51,66,69). The relationship between colonization by H. pylori and the onset of the disease is not fully understood. Hence, it is important to identify essential bacterial virulence factors and elucidate their contribution to disease development.Several virulence factors contribute to the stringent host and tissue specificities exhibited by H. pylori (37). Among them, urease helps neutralize the acidic pH surrounding the bacteria and allows their survival in the gastric environment (21, 45). In addition, the spiral shape and unipolar flagella of H. pylori confer on the bacterium a corkscrew motion that enhances motility in the viscous gastric mucus (32, 33, 63) and is essential for host colonization (22,23,35). Lipopolysaccharide (LPS) is also important for the virulence of H. pylori since strains lacking the O antigen are significantly impaired in their capacity to colonize the murine stomach (40). The H. pylori O antigen is composed of N-acetyl-D-glucosamine, L-fucose, and D-galactose (4, 5, 46), which form structural motifs that are identical to human blood group antigens Lewis X, Y, and b (4,5,[46][47][48]....
