Challenge of LT-HSCs (LKS+ CD105+) with C. albicans yeast also induces their proliferation as well as the upregulation of myeloid INCB018424 manufacturer progenitor markers (CD34 and FcγR) through a TLR2/MyD88-dependent signaling pathway. TLR2/MyD88 signaling also promotes, upon challenge with yeast or Pam2CSK4, the differentiation of CMPs and GMPs into cells with a morphology of mature myeloid cells expressing
CD11b, F4/80, and Gr-1. These myeloid-like cells display functional properties, as they are able to (i) phagocytose C. albicans yeast and (ii) produce proinflammatory cytokines upon stimulation [42]. The specific myeloid subsets that are produced following in vitro exposure of mouse HSPCs (Lin− cells) to C. albicans have been also determined. Inactivated C. albicans yeast induced
the differentiation of monocyte-derived DCs (moDCs, CD11bhigh CD11c+ Ly6C+ F4/80+) via TLR2/MyD88- and Dectin-1-dependent pathways. Interestingly, the response to C. albicans yeast was more similar to the response to curdlan (a pure Dectin-1 ligand) than to Pam2CSK4 (a pure TLR2/TLR6 ligand), as Pam2CSK4 promoted differentiation to macrophages (CD11bhigh CD11clow Ly6C+ F4/80high) rather than moDCs [26], indicating that Dectin-1 plays a key role in the response to C. albicans. Dectin-1 is not expressed on the most primitive stem cells, the “side see more population” cells, but a subset of Lin− cells express detectable levels of Dectin-1 [26], indicating that it is turned on in differentiating progenitors prior to
the acquisition of lineage markers. The moDCs generated in vitro, in response to inactivated yeasts, are functional as they have acquired the capability to secrete TNF-α and have fungicidal activity, and therefore could participate Selleck Rucaparib in innate immunity against C. albicans. All these data strongly support the notion that TLR signaling programs early progenitors to generate functional mature cells to deal with the fungal pathogen (Fig. 2). Direct in vivo interaction of pathogens and/or their components with TLRs on HSPCs during infection is more difficult to demonstrate. As noted above, HSPCs in an intact mouse could also respond to other stimuli, including inflammatory cytokines generated by differentiated cells responding to the infection, such as TLR-expressing tissue macrophages or epithelial cells [12, 38, 43]. For instance, it is well established that cytokines such as IFNs (IFN-α, IFN-β, and IFN-γ) and TNF-α play an essential role in HSPC proliferation in response to infection [7, 8, 44]. However, it has been recently shown that IFN-γ impairs proliferation of HSCs in mice by acting as a negative modulator of HSC self-renewal [28], so the role of IFN-γ in quiescent HSCs remains to be clearly established.