Together, these data suggest a novel mechanism of immunosuppression by dexamethasone. To induce immune synapse formation, untransformed resting human peripheral blood (PB) T cells were incubated with superantigen (Staphylococcus aureus enterotoxin B, SEB) loaded APCs. The immune synapse formation was analyzed using multispectral imaging flow cytometry (MIFC), which combines fluorescence click here microscopy and flow cytometry. MIFC allows the spatial quantification of fluorescence signals within T cells by defining regions of interest for the measurement (Supporting Information Fig. 1). T-cell/APC couples were identified by gating on cell clusters
according to DNA content (Hoechst33342 staining) and CD3 expression (Fig. 1A, blue gate). T-cell/T-cell couples (Fig. 1A, green gate) or cell clusters that contained more than one T cell or APC (Fig 1A, black gate) were eliminated from further analysis. Then, the accumulation of the TCR/CD3 complex and LFA-1 in the T-cell/APC contact zone was used as measure for immune synapse formation. As expected, in the absence of superantigen most T cells did not show an enrichment of TCR/CD3 and LFA-1
in the contact zone (Fig. 1B, left side). DAPT in vivo In the presence of SEB, however, T cells showed a clear formation of an immune synapse (Fig. 1B, right part). To quantify the number of T cells with an immune synapse, we acquired up to 25 000 T cells. Figure 1C shows the frequency of primary human T cells that showed an enrichment of TCR/CD3 and LFA-1 in the contact zone from 19 different donors. The mean number of
T cells with an immune synapse increased significantly in the presence of SEB. It is important to note that the variations of T cells forming immune synapses were relatively high between different donors, ranging from 0.2 to 1.5% (Fig. 1C). We therefore compared the values from experiments that were performed in triplicates to evaluate the variance in dependent samples (Fig. 1D). The mean standard deviation of the triplicates Histamine H2 receptor (intratest SD) was 7.5 per 10 000 T cells. Taken the high variations between different donors (Fig. 1C) and the low variations of the triplicates (Fig. 1D) into account, we decided to normalize the following experiments by setting the numbers of T cells of one individual with synapses in the absence of dexamethasone as 1. To analyze the effects of glucocorticoids on the formation of an immune synapse in untransformed human T cells, PB T cells were preincubated with the glucocorticoid dexamethasone (5 μM). This concentration inhibited blast formation and cell-cycle entry without having any toxic effects (Supporting Information Fig. 2). Interestingly, in dexamethasone pretreated T cells, an inhibition of TCR/CD3 and LFA-1 accumulation and thus immune synapse formation could be observed (Fig. 2A and B). The reduced maturation of the immune synapse was due to a combined failure of LFA-1 (Fig. 2C) and CD3 (Fig.