These data point to IL-2 signaling as another target for zinc in T cells, in addition to TCR signaling. Upon stimulation, the IL-2-receptor (IL-2R) activates signal transduction pathways, including STAT5 and ERK1/2. The β- and γ-chains of the IL-2R are associated with

JAK1 and 3, which transphosphorylate each other and subsequently the β receptor-chain at the key positions Tyr338, Tyr393, and Tyr51010. Phosphorylation of these tyrosines forms binding sites for the SH2-domain of STAT5, which becomes activated by JAK via phosphorylation selleck chemical of Tyr694, leading to dimerization to a transcription factor that promotes transcription of genes such as c-myc, bcl-2, CD25, and bcl-x 11. Additional feedback regulation of this pathway occurs via SOCS and cytokine

Dorsomorphin ic50 inducible SH2-containing protein (CIS) 12. MAPK transduce extracellular signals from hormones, growth factors, cytokines, and environmental stress, thereby regulating a variety of cellular responses including cell proliferation, migration, differentiation, and apoptosis 13. Phosphorylation of Tyr338 of the IL-2R β-chain leads to the assembly of adaptor proteins SHC, Grb2, and SOS1. This triggers a MAPK-cascade consisting of the dual-specific kinases RAF and MEK, which activates ERK via phosphorylation of conserved tyrosine and threonine residues in its catalytic domain 10. Upon activation, ERK phosphorylates several other kinases and activates Vasopressin Receptor transcription factors, such as c-fos, c-jun, elk-1, and c-myc 14. Negative regulation of the ERK pathway is mediated by various phosphatases, including several dual specificity Thr/Tyr protein phosphatases (DUSP) and protein phosphatase 2A (PP2A) 13. Here, we demonstrate that IL-2 induces a zinc signal, i.e. a

translocation of zinc ions from lysosomes into the cytosol. This signal is required for inhibition of ERK dephosphorylation and IL-2-induced T-cell proliferation, but has no effect on STAT5 signaling. Upon staining of the murine cytotoxic T-cell line CTLL-2 with the zinc-selective fluorescent probes Zinquin and FluoZin-3, we found differential intracellular localization of the probes (Fig. 1A). Zinquin showed a relatively uniform staining throughout the entire cell, whereas FluoZin-3 exclusively labeled vesicular structures. These so-called zincosomes sequester high amounts of zinc 15. After stimulation with IL-2, intracellular translocation of zinc occurred (Fig. 1B and C; Supporting Information Fig. 1A). Vesicular FluoZin-3 fluorescence decreased in response to IL-2. In contrast, an increase of the cytoplasmic zinc-dependent fluorescence was measured with Zinquin. There were no major differences in the intracellular localization of the fluorescence before and after treatment with IL-2, indicating that IL-2 affects the intensity of zinc staining in the different compartments, rather then the distribution of the fluorescent dyes (Supporting Information Fig. 2).