Groups of mice immunized by the intranasal or intravenous route with either OVA and α-GalCer (α-GalCer group) or OVA alone (control group) were sacrificed on days 1, 3, 5, 6, 8, and 10 post-immunization (Fig. 1A). A second (booster) immunization was delivered in each case to additional groups of mice on day 5 and sacrificed on days 6, 8, and 10 (i.e. days 1, 3, and 5 respectively, relative buy Crizotinib to the second dose). Single-cell suspensions prepared from spleen and lung tissues were analyzed for functional activation of NKT
cells in terms of IFN-γ production (Fig. 1B). We observed a significant increase in the number of IFN-γ-producing NKT cells after intranasal immunization in mice from the α-GalCer group, relative to that in the control group animals, with peak activity at one day after the first as well as the second dose. In contrast to these results, mice immunized by the intravenous route showed a significant beta-catenin inhibitor increase in the number of IFN-γ-producing NKT cells at day one after only the first dose, and not the second dose (Fig. 1C). These results from mice immunized by the intravenous route are consistent with the reports in the literature showing that a single dose of systemic
α-GalCer administered either by the intravenous or intraperitoneal route induced NKT cell anergy, where NKT cells become unresponsive to a second or booster dose of α-GalCer administered by the same route, in terms of an inability to produce IFN-γ or proliferate 5, 6, 8, 9. Along
with increased IFN-γ production, expansion of NKT cells also occurred in the α-GalCer group with the peak levels observed at day 5 after the priming immunization by the intranasal route in the lung (Fig. 1D). Of importance is the observation of a second wave of expansion of the NKT cells in the lung between days selleck 6 and 10 (i.e. days 1 and 5 respectively, after the second intranasal immunization) that is significantly higher when compared with the percentages of NKT cells at the corresponding time point in the mice that did not receive the second immunization or the control group of mice that received two doses of OVA only (Fig. 1D). In the mice immunized by the intravenous route with two doses of α-GalCer, there was a slight increase in the NKT population at day 8, which corresponds to day 3 post-boost (Fig. 1D); however, this increase was smaller and less sustained than what was observed in the intranasal group and did not correspond to increased IFN-γ production (Fig. 1C). The reactivation of NKT cells paralleled an increase in the CD86 expression on CD11c+ DCs (Fig. 2A and B) in the spleen and lung after the second intranasal dose of α-GalCer+OVA when compared with the OVA control group on day 1 after the second immunization, a trend similar to that observed for activation of DCs on day 1 after the primary immunization (Fig. 2A and B).