Abstract
Dendritic epidermal T cells (DETCs) represent a prototypical lineage of intraepithelial γδ T cells that participate in the maintenance of body barrier homeostasis. Unlike classical T cells, DETCs do not recirculate and they remain persistently activated through their T cell receptors (TCR) at steady state, i.e., in absence of infection or tissue wounding. The steady state TCR signals sustain the formation of immunological synapse-like phosphotyrosine-rich aggregates located on projections (PALPs) which act to anchor and polarize DETC’s long cellular projections toward the apical epidermis while the cell bodies reside in the basal layers. The PALPs are known to contain pre-synaptic accumulations of TCR-containing and lysosomal granules, but how this cargo accumulates there remains unclear. Here, we combined anti-Vγ5 TCR, cholera toxin subunit B (CTB), and LysoTracker (LT)-based intravital labeling of intracellular granules, with high resolution dynamic microscopy and fluorescence recovery after photobleaching (FRAP) to characterize the steady state composition and transport of DETC granules in steady state epidermis. Intradermal fluorescent Vγ5 antibody decorated DETCs without causing cellular depletion, dendrite mobilization or rounding up and became slowly internalized over 48 h into intracellular granules that, after 6 days, colocalized with LAMP-1 and less so with LT or early endosomal antigen-1. Intradermal CTB was likewise internalized predominantly by DETCs in epidermis, labeling a partly overlapping set of largely LAMP-1+ intracellular granules. These as well as LT-labeled granules readily moved into newly forming dendrites and accumulated at the apical endings. FRAP and spatiotemporal tracking showed that the inside tubular lengths of DETC cellular projections supported dynamic trafficking of lysosomal cargo toward and away from the PALPs, including internalized TCR and lipid raft component ganglioside GM1 (labeled with CTB). By contrast, the rate of GM1 granules transport through comparable dendrites of non-DETCs was twice slower. Our observations suggest that DETCs use chronic TCR activation to establish a polarized conduit system for long-range trans-epithelial transport aimed to accumulate mature lysosomes at the barrier-forming apical epidermis. The biological strategy behind the steady state lysosome polarization by DETCs remains to be uncovered.
Highlights
Considered a member of the innate body barrier defense system, murine dendritic epidermal T cells (DETCs) contribute to skin repair and homeostasis [1,2,3]
We described the in vivo phenomenon of DETC steady state apical polarization through the dendriteterminal T cell receptors (TCR) activation in the phosphotyrosine-rich aggregates located on projections (PALPs) [5]
This study follows upon the discovery of DETC in vivo trans-epidermal polarization through the steady state TCR activation in the PALPs [5]
Summary
Considered a member of the innate body barrier defense system, murine dendritic epidermal T cells (DETCs) contribute to skin repair and homeostasis [1,2,3]. These cells extend long cellular processes from the mid-body in the basal epidermis toward the apical epidermis thereby spanning across the whole epidermis thickness and interacting with both the immature (basal) and mature (squamous) keratinocytes. The dendrite-terminal cytoplasm underneath the PALPs harbors distinct accumulations of intracellular granules some of which contain TCR and/or lysosomal and exocytic pathway markers LysoTracker (LT), GM1, and LAMP-1 [5]. The in vivo behavior of DETC’s intracellular cargo has remained unknown
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