On day 6, the NF-κB inhibitor-treated and -untreated im-DCs were incubated with LPS or TNF-α to see if they could be induced to mature. Comparative study of the expression of surface molecules on LPS-induced mature DCs (m-DCs) that might be related to allostimulation found that AZM, added at 50 µg/ml on days 0, 3 and 6, inhibited the expression of MHC class II

and co-stimulatory molecules (CD40, CD80 and CD86) when Vit. D3 was used as a positive control [30] (Fig. 1a). Conversely, the PPAR-γ activator, ACE inhibitor and clarithromycin did not suppress the expression of MHC class II or co-stimulatory molecules (Fig. 1a). When the expression levels were compared on the basis of the mean fluorescence intensity (MFI), the expression of MHC class II and co-stimulatory molecules but not CD80 were decreased significantly in a dose- and time-dependent manner (Table 1). TLR-4 INK 128 cost Copanlisib order expression was also decreased in AZM-treated im-DCs stimulated with TNF-α (Fig. 1b). The MFIs of TLR-4 of

control m-DCs and AZM-treated m-DCs were significantly different (13·39 ± 1·07 versus 8·56 ± 0·47; P < 0·01, n = 3) (Fig. 1b). Similar to the results for expression of MHC class II and co-stimulatory molecules, the PPAR-γ activator, ACE inhibitor and clarithromycin did not affect expression of TLR-4 (Fig. 1c). We also confirmed that the vehicles used to dissolve the NF-κB inhibitors 4��8C did not affect the expression of these antigens and showed no toxicity when we added equal amounts of them to culture wells as controls (data not shown). Morphologically, AZM-treated im-DCs (Fig. 1d) were similar to control im-DCs

(Fig. 1e). However, in the case of LPS-induced m-DCs, AZM treatment resulted in less prominent dendrite formation, with a round nucleus (Fig. 1f), compared with the control cells (Fig. 1g). To determine whether AZM might affect the functions of DCs, we first compared IL-12p70 production by AZM-treated and -untreated im-DCs stimulated with LPS. As shown in Fig. 2a, the IL-12p70 concentration was significantly lower in the supernatant of AZM-treated im-DCs (P < 0·001). We next asked whether AZM might affect the allogeneic T lymphocyte stimulatory capacity of DCs. To address this question, we performed MLR experiments. [3H]-Thymidine incorporation was suppressed significantly when allogeneic T lymphocytes were stimulated with m-DCs treated with 50 µg/ml of AZM, causing up to 27% reduction of the allostimulatory capacity (Fig. 2b). We also investigated the secretion levels of IFN-γ and IL-10 in the MLR supernatant by enzyme-linked immunosorbent assay. IFN-γ was reduced by 31% when allogeneic T lymphocytes were stimulated with AZM-treated m-DCs compared to untreated m-DCs, indicating that AZM-treated m-DCs decreased Th1 polarization (Fig. 2c).