Thioredoxin activity of rHBP35 proteins Shiroza et al. [12] have shown that an hbp35 gene-containing plasmid complemented the defects in motility SU5402 cost and alkaline phosphatase activity of an E. coli dsbA mutant. This finding indicates that HBP35 is exported to the periplasm in a dsbA mutant and plays a role in the disulfide bond formation [13]. The HBP35 protein has a thioredoxin motif in
the N-terminal region. We performed an insulin reduction assay to determine whether HBP35 has thioredoxin activity. Reduction of disulfide bonds of insulin by thioredoxin activity generates free A and B chains of insulin, and the resulting B chain is precipitated, which can be measured by the increase in turbidity [14]. The reducing activity of rHBP35 (Q22-P344) was higher than that of STA-9090 price E. coli thioredoxin, whereas no activity was detected in rHBP35 (Q22-P344
with C48S and C51S), indicating that HBP35 protein exhibits thioredoxin activity and that the two cysteine residues (C48 and C51) are crucial for this activity (Figure 6). Figure 6 Thioredoxin-catalyzed reduction of insulin by DTT. Increase in turbidity at 650 nm was plotted against reaction time. Closed diamond, rHBP35(Q22-P344) plus DTT; closed square, E. coli thioredoxin plus DTT; closed triangle, rHBP35(Q22-P344 with C48S C51S) plus DTT; X, rHBP35(Q22-P344) without DTT. Diffuse bands of 50-90 kDa proteins are associated with selleck kinase inhibitor anionic polysaccharide Nguyen et al. [11] revealed glycosylation of RgpB by immunoblot analysis with a Fenbendazole monoclonal antibody (MAb 1B5) that recognizes the anionic polysaccharide of A-LPS [10, 15]. To determine whether
HBP35 is glycosylated, we carried out an immunoprecipitation experiment. Immunoprecipitates from the protein extracts of KDP136 (gingipain-null mutant) with an anti-HBP35 rabbit polyclonal antibody contained the 40-kDa protein and diffuse proteins of 50-90 kDa, which were revealed by immunoblot analysis with an anti-HBP35 mouse monoclonal antibody (MAb Pg-ompA2) [16]. The diffuse proteins of 50-90 kDa immunoreacted with MAb 1B5, indicating that HBP35 is associated with anionic polysaccharide on the cell surface (Figure 7). It is likely that the diffuse bands are HBP35 proteins binding to anionic polysaccharides with different numbers of repeating units. Figure 7 Posttranslational glycosylation of HBP35 in P. gingivalis KDP136 (gingipain-null mutant). Immunoprecipitates with anti-HBP35 antibody (lane 1), with anti-Dps antibody (lane 2), and without an antibody (lane 3) were loaded on SDS-10% polyacrylamide gel and immunoblot analysis was performed with MAb Pg-ompA2 (A), MAb 1B5 (B), and anti-Dps antibody (C).