The correlation between the antibody concentration in sera and intestinal washes in each animal was performed calculating the Pearson’s correlation coefficient r. The lymphoproliferative response between groups was analyzed using one-way
ANOVA and Tukey’s post test. Statistical significance was defined as P ≤ 0.05. Graphpad 4.0 software was used for analysis. Vi-specific serum GSK1210151A ic50 antibodies were assessed in mice subcutaneously immunized with Vi-CRM197, unconjugated Vi, free CRM197 or PBS. Two weeks after priming (day 13), both Vi-CRM197 and Vi immunized mice developed a significant serum Vi-specific IgM response with a geometric mean titer [GMT] of 1280 and 425 respectively (P < 0.001 versus PBS immunized mice; Fig. 1A and Table S1). IgM titers induced by the glycoconjugate were significantly higher than those observed in Vi immunized mice (P < 0.01) ( Fig. 1A and Table S1). After boosting, Vi-specific IgM significantly selleck kinase inhibitor decreased (P < 0.05) while IgG significantly increased in Vi-CRM197-immunized mice (GMT of 1689 after priming [day 13] and of 4560 after boosting [day 24], P < 0.01) and persisted until day 60 with titers
significantly higher compared to mice immunized with Vi or CRM197 alone (P < 0.001; Fig. 1B and Table S2). In Vi-immunized mice the IgG response did not significantly increase after boosting, and persisted up to day 60 with a GMT of about 256 (P < 0.001 versus
PBS and CRM197 groups; Fig. 1B and Table S2). The IgG response detected in mice immunized Astemizole with Vi-CRM197 was about 8 times higher than that induced by unconjugated polysaccharide Vi after the primary immunization and about 18 times higher after boosting. These data demonstrate that the glycoconjugate was more efficient in stimulating antibody isotype switching. The analysis of Vi-specific serum IgG subclasses 10 days after boosting (day 24) showed a predominance of IgG1 in mice immunized with Vi-CRM197 (P < 0.001 versus other subclasses; Table S3) that were significantly higher than those observed in mice immunized with Vi antigen alone (P ≤ 0.001; Fig. 1C). These data corroborate the IgG subclass switch observed with other polysaccharides, such as pneumococcal and meninogococcal polysaccharides and their respective conjugate vaccines [13], [14] and [15]. No significant levels of serum Vi-specific IgA were detected in any group. Mice immunized with Vi-CRM197 developed a CRM197-specific serum IgG response with a subclass distribution similar to that observed for anti-Vi IgG (data not shown). This work therefore shows that boosting with Vi-CRM197 induces a significant increase of serum IgG typical of secondary antibody response to T-dependent antigens, and a dominance of the IgG1 subclass.