2b) IgM increased significantly only in the D-LL + Lc (N) group

2b). IgM increased significantly only in the D-LL + Lc (N) group compared to LL (P < 0·05) and LL + Lc (0), but only on day 28 (P < 0·05) (Fig. 2c). The levels of IgA in serum showed no significant differences among the different groups assayed (Fig. 2a). In order to study whether the specific humoral immune response

induced by the different immunization strategies used in this work increased resistance in mice against a pneumococcal infection, the animals were challenged intranasally with serotypes 3 and 14 of the pathogen. Analysis of the infection was carried out evaluating colonization in lung and pathogen passage into blood on day 2 after challenge (Table 2). All the treatments prevented colonization CP-690550 clinical trial in lung by both S. pneumoniae

serotypes and also prevented dissemination into the BGB324 datasheet blood of serotype 14. In contrast, when animals were infected with serotype 3, only administration of the recombinant bacterium, live (LL) and dead (D-LL), associated with the oral administration of the probiotic strain Lc, prevented dissemination of the pathogen into the bloodstream. Administration of D-LL + Lc (N) did not prevent colonization of the lung by serotype 3. These results demonstrate that immunization with LL + Lc (O) and D-LL + Lc (O) would be the most effective treatment for the prevention against pneumococcal infection of young mice with S. pneumoniae. The effect of different

treatments on the vaccine-induced immune response is important in the selection of a vaccination strategy adequate against a specific pathogen. We assessed the levels of IgG1 and IgG2a anti-PppA post-vaccination (day 42) in order to analyse the Th1/Th2 balance in both BAL and serum. Th1 cells secrete IFN-γ, associated with switching to IgG2a, while Th2 cells secrete mainly IL-4, which promotes switching to IgG1. The results obtained are shown in Table 3 and correspond to the IgG1/IgG2a ratio for each group on day 42 (2 weeks after the third immunization). Administration of LL induced a mixed-type Th1/Th2 response in BAL. The live vaccine associated with the oral administration of Lc [LL + Lc MYO10 (O)] and the inactivated vaccine (D-LL) induced a significant increase in the IgG1/IgG2a ratio, indicating preferential activation of Th2 cells. In contrast, immunization with D-LL + Lc (N) and D-LL + Lc (O) showed a significant decrease in the IgG1/IgG2a ratio compared to the other groups. This would indicate that the probiotic would induce a shift towards the type Th1 response. Similar results were found in serum, although the LL + Lc (O) group did not show significant differences with LL. The type of immune response induced in the respiratory mucosa is decisive in the protection of the host against pathogens that enter the organism through the airways.

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