CpG ODN is a ligand for TLR9 and therefore was not expected to signal through TRIF because TLR9 signals exclusively via the MyD88-dependent pathway. As discussed above, TLR4, for which LPS is a ligand, utilizes either MyD88 or TRIF as adaptor molecules. In this case it appeared that the observed effects were diminished by deletion of either MyD88 or TRIF, but that the effect of MyD88 deletion was more marked. From this data it was concluded that signalling through both the MyD88-dependent and the MyD88-independent/TRIF-dependent pathways could initiate
changes in lineage commitment in developing haematopoietic cells in vitro, which was dependent on the inducing ligand. The data from experiments involving influenza viruses demonstrated that, although they have been shown to activate MyD88-dependent signalling in B lymphocytes, https://www.selleckchem.com/products/ensartinib-x-396.html in this instance their effects were INCB024360 ic50 mediated by a mechanism that was not dependent on either MyD88 or TRIF. As the above evidence demonstrated that the effects of LPS on BMDC generation were dependent, in part, on both MyD88 and TRIF, and LPS has been shown to be a ligand for TLR4,16 which interacts with both adaptors, it was important to directly confirm the role of TLR4 in modulating the effects of LPS on BMDC production in vitro. To assess this, bone marrow cells from C57Bl/6 (TLR4+/+) and TLR4−/− mice were cultured in the presence of GM-CSF, with or without Poly I, Poly I:C, LPS or CpG, for 6 days. The
production of BMDCs was assessed by monitoring the surface expression of CD11c and MHCII. The results (Fig. 4) confirm a requirement for TLR4 in signalling initiated by LPS. Stimulation of TLR4+/+ bone marrow cultures with Poly I, Poly I:C, LPS or CpG resulted in a striking reduction in the production of CD11c+/MHCII+ BMDC, similar to that observed in BALB/c bone marrow cultures. A similar reduction in BMDC production was observed in cultures of TLR4-deficient bone marrow containing Poly I, Poly I:C or CpG. By contrast, TLR4-deficient bone marrow cultures containing LPS displayed a level of BMDC production comparable to that observed in unstimulated
cultures. This evidence supports the previous findings that MyD88 and TRIF are involved in signalling downstream from LPS and confirms a role for TLR4 in regulating changes in BMDC production. Type A influenza viruses have been shown to be strong inducers PJ34 HCl of type 1 IFNs,17 which are a major component of the antiviral response, inducing an antiviral state in uninfected cells18. It therefore seemed possible that the effects seen in our experiments in response to influenza A viruses could be mediated by type 1 IFNs. To investigate this we first examined the effects of influenza viruses on the generation of BMDCs in cultures of bone marrow cells from IFNAR−/− and IFNAR+/+ mice in the presence of GM-CSF. Cultures containing IFNAR+/+ bone marrow cells displayed reduced CD11c+/MHCII+ BMDC production in response to the addition of Jap, X31 or PR8 virus (Fig.