7D). These results suggest that galectin-3 might not directly affect the in vitro differentiation of TREG cells, but reinforces a critical role for this lectin in the control of IL-10 production and modulation of Notch activation. In the present study, we identified a role for endogenous galectin-3

as a negative regulator of TREG cell frequency and function during L. major infection. Moreover, our results show that endogenous galectin-3 selectively influences downstream molecular targets Selleckchem Inhibitor Library including IL-10 and Notch signaling. Galectin-3 is an immunoregulatory lectin widely distributed in different tissues including sites of inflammation and infection [1, 23] and modulates the fate and function of different cell types [5, 24, 25]. With regard to T cells, galectin-3 is expressed by activated but not resting CD4+ and CD8+ T cells [25]. Although different groups have reported several roles for exogenous and endogenous galectin-3 in T-cell activation, differentiation, and apoptosis [26, 27], the function of this lectin within the TREG-cell compartment is largely unknown. We found increased percentage of peripheral TREG cells in noninfected Lgals3−/− compared with WT mice. Remarkably, the frequency of TREG cells at infection sites and draining LN was significantly BIBW2992 concentration increased during chronic leishmaniasis

in Lgals3−/− mice compared with WT mice. Several possibilities may explain this phenomenon, including selective attraction of TREG cells by tolerogenic DCs present in secondary lymphoid organs and infected tissues [28] and/or active proliferation of TREG cells in vivo following antigenic stimulation [29]. Given our previous observations that galectin-3 has inhibitory Mirabegron effects on IL-12 production by DCs [5], the increased activation of DCs from Lgals3−/− mice could lead to enhanced migration

of TREG cells to sites of infection. In addition, TREG cell homing is dictated by the expression of cell adhesion molecules, including CD103 [17] and CD62L [30], which regulate their tissue-specific trafficking, recruitment, and function. Our findings show that draining LNs from Lgals3−/−-infected mice contains higher frequency of TREG cells, which display increased expression of CD103. Whether endogenous galectin-3 could affect TREG-cell recruitment via CD103-mediated mechanisms remains to be elucidated. Alternatively, as expression of CD103 is upregulated by TGF-β [31], the higher production of TGF-β by Lgals3−/− TREG cells could also account for the upregulated expression of this molecule. In the past few years, new findings have challenged the classical Th1/Th2 paradigm in mice “resistant” and “susceptible” to L. major infection. These findings revealed that IL-10 is one of the crucial factors responsible for the susceptibility to L. major infection, besides the traditional IL-4R pathway [32-34]. In L.