Co-localisation of AIRE with cytoskeletal filaments was also observed in some cells as previously been reported in Aire-transfected cell lines 36–38. All non-transduced cell lines failed to stain for AIRE, suggesting that the endogenous AIRE expression was
lacking or at undetectable levels (Fig. 1B). AIRE expression, as assessed by flow cytometry was maintained in GFP+ cells even after several passages in cell culture (Fig. 1C). GFP+ cells continued to grow well in culture without any obvious adverse effect on doubling time or survival. Having established this panel of AIRE-expressing cell lines, we asked whether AIRE expression was sufficient to activate the expression of a panel of TRA; thus, potentially mimicking the role of AIRE in the thymus. The TRA selected Carfilzomib supplier for quantitative RT-PCR (qRT-PCR) represented autoantigens associated with defined autoimmune diseases such as type 1 diabetes (Ins2), EAE/MS (Mbp, Mog, Plp1), autoimmune gastritis (Atp4a), hypothyroidism (Nalp5), uveitis (Rbp3) and Sjögren’s syndrome (Spt1). Spna2 (α-fodrin) was included as a negative control, and although identified as a target autoantigen
in Sjögren’s syndrome-like pathology in Aire−/− mice, its expression in the thymus is independent of AIRE 18. Corroborating immunofluorescence studies, Aire transcript levels in transduced cell lines were at least 10 000-fold above non-transduced cells (Fig. 2A). As predicted, Spna2 expression was unaltered across the cell lines. We observed that the level of TRA mRNA modulation check details was not consistent across the different cell lines. The transduced thymic derived cell lines (B6TEA and 427.1) expressed a greater number of TRA in comparison with other cell lines tested; however, the expression of specific TRA differed
between these lines Liothyronine Sodium (Fig. 2A). For example, Mog was highly upregulated in transduced 427.1 cells but was unaltered in B6TEA cells, whereas the expression of another myelin antigen gene, Mbp, was upregulated in B6TEA, but was unaffected in 427.1 cells. Further highlighting this heterogeneity was the observation that Atp4a displayed higher expression in B6TEA and 427.1 thymic epithelial cell lines compared with the macrophage (J774 and RAW267.4) and fibroblast lines (Fig. 2A). Given the relatively high expression of Mog we observed in 427.1 cells we examined these cells for MOG protein expression using an anti-MOG specific monoclonal antibody 29. Aire-transduced cells expressing GFP (and thus AIRE) were specifically reactive with the anti-Mog monoclonal antibody, confirming that the expression of AIRE in these cells promotes MOG expression (Fig. 2B). Non-transduced 427.1 did not display any MOG reactivity, and staining of control cells (NIH/3T3) transduced with retrovirus encoding Mog demonstrates the specificity of the anti-Mog monoclonal antibody in transduced (GFP+) cells (Fig. 2B).