A wealth of information has been amassed regarding the localization of signalling molecules, their kinetics and the transcription factors click here they activate. We continue to discover mechanisms that cause receptors and signalling molecules to compartmentalize in the cell; however, the emerging challenge lies
in understanding how the immunological synapse contributes to differentiation. Here, we review some of the transcription factors activated downstream of T-cell receptor signalling and discuss mechanisms by which antigen dose and affinity may influence differentiation. Antigen affinity might change the kind of transcription factors that are activated whereas antigen dose is likely to influence the temporal dynamics of the transcription factors. The immunological synapse is therefore likely to influence differentiation YAP-TEAD Inhibitor 1 by modulating the trafficking of transcription factors and by promoting asymmetric cell division, an emerging concept. The term immunological synapse was first proposed by Paul and Seder as a cognate interaction of a T cell and an antigen-presenting B cell which the T cell uses to secrete effector cytokines in the synaptic cleft to cause humoral responses.1 Kupfer and colleagues were first to define the compartmentalization of interactions at
the interface of T and B cells as the central accumulation of T-cell receptor–major histocompatibility complex–peptide (TCR-MHCp) interactions surrounded by a peripheral ring of adhesion molecule interactions. They called these zones central and peripheral supra-molecular activation clusters, respectively (c-SMAC
or p-SMAC). In the context of the synapse they found that protein kinase C-θ (PKC-θ) was localized to the c-SMAC whereas Talin, a molecule known to modulate adhesion, was localized to the p-SMAC.2 The kinetics of synapse formation was first demonstrated by Grakoui et al.3 Using glass-supported planar lipid membranes incorporated with lipid-anchored peptide–MHC complexes and intercellular adhesion molecule 1, it was demonstrated that immediately after contact initiation TCR-MHCp interactions are largely in the periphery next and the adhesion interactions are in the centre. Within a few minutes, there is a re-organization of these interactions to form the mature synapse. The impacts of antigen dose, affinity and the role of the co-receptor CD4 were also examined in these studies.3 The immunological synapse is also the site for signal initiation and integration.4–6 This paradigm has been effective in conveying an understanding of the spatial and temporal dynamics of proximal signalling (see Fig. 1) components over short time-scales of minutes to an hour. Differentiation of T cells, however, takes place over days, and although several distinct environmental signals contribute to differentiation, TCR signals remain central to this differentiation process.