In the murine system, immune synapses can be analyzed in vitro using TCR transgenic
T cells and supported planar bilayers (e.g. 2, 18), or APCs loaded with the cognate antigen Histone Methyltransferase inhibitor 19–21. Intravital microscopy in mice even allows analysis of T-cell/APC contacts in their physiological environment, e.g. in LNs 22–24. However, with regard to L-plastin regulation and function, clear differences exist between mice and human. Thus, the activation-induced upregulation of the surface receptors CD25 and CD69 is dependent on L-plastin phosphorylation in human T cells 8, but expression of this protein seems to be dispensable for activation-induced CD69 upregulation in murine T cells 25. The analysis of immune synapses of T cells of human origin has also been performed in Jurkat T-lymphoma cells 26–28. However, Jurkat T cells display strong distinctions from primary human T cells in their signaling pathways. For example, PI3K is a downstream effector of Ras in primary human T cells 29,
but not in Jurkat T cells 29, 30, which might, e.g., be due to a defective expression of the phosphatase PTEN in Jurkat T cells 31. Therefore, all experiments presented here were performed with primary human T cells. This research is challenging because primary human T cells represent a heterogeneous cell population in which only a small fraction of cells reacts on a given antigen, which limits the number of T-cell/APC couples to be evaluated 5, 26, 32, 33. Recent proceedings in high-throughput imaging significantly improved the statistical
evaluation click here of receptor clustering in the immune synapse of primary T cells 5, 16. Using such a high-throughput ImageStream™, we show here for the first time that dexamethasone interferes with actin stabilization and prevents the formation of the immune synapse of untransformed human T cells. Immune synapse formation requires Urocanase a dynamic reorganization of the actin cytoskeleton. During the reorganization process, G-actin is polymerized to F-actin by the Arp2/3 complex. The existing actin fibers are then dynamically depolymerized by cofilin or stabilized by actin crosslinking or bundling proteins (for review, see 6, 17). Here, we show that the phosphorylation of the actin-bundling protein L-plastin on Ser5, which represents a costimulatory signal 8, 9, is inhibited by dexamethasone. Nevertheless, although it was known that glucocorticoids can modify the actin cytoskeleton in endometria cells 34 or stabilize F-actin in AtT-20 cells 35, the targets of glucocorticoids that are involved in actin cytoskeleton changes were unknown. The inhibition of L-plastin phosphorylation upon costimulation of primary human T cells is therefore the first known event that may explain the effects of dexamethasone on the actin cytoskeleton. In order to get fully activated, T cells require costimulation, i.e.