How IL-21 promotes pathogenesis of T1D is not yet clear. IL-21 is produced mainly by natural killer

(NK) T cells and CD4+ T cells [12, 13]. All CD4+ T helper subsets can produce varying amounts of IL-21, depending on the context of stimulation and the cytokine milieu [14, 15]. Crizotinib IL-21 acts as an autocrine growth factor that shifts the balance away from Tregs towards the T helper type 17 (Th17) lineage, promoting inflammation and immune response [16, 17]. In psoriasis and multiple sclerosis Th17 cells, driven partly by IL-21, play a significant role in promoting tissue damage [18-20]. Early studies in NOD mice lacking IL-21Rα have also implicated IL-21 in T1D pathogenesis via Th17 cells [8, 15]. However, the role of Th17 cells in the pathogenesis of T1D remains controversial. In fact, Th17 cells produced in the

gut have been shown to exert a protective effect in T1D [21-25]. CD8+ T lymphocytes play a key role in the pathogenesis of autoimmune diseases by causing damage to target organs [26]. Two recent studies have implicated IL-21 in T1D pathogenesis via promoting expansion and survival of CD8+ T cells [9, 11]. Studies on the role of IL-21 in viral infections showed BMN 673 clinical trial that IL-21 signalling is indispensable for robust primary and secondary CD8+ T cell responses to chronic viral infections [27-31]. These studies suggested that IL-21 may also be needed for the efficient activation of autoreactive CD8+ T cells. This possibility is supported by our recent finding that IL-21, in synergy with IL-15, enables naive autoreactive CD8+ T cells to respond

to weak TCR agonists and induce disease in an engineered model of T1D [32]. In the present study, we have examined click here the role of IL-21 in activating autoreactive CD8+ T cells in the NOD mouse expressing the transgenic 8.3 T cell receptor (TCR) [33]. Our findings indicate that IL-21 is required for the initial activation of autoreactive CD8+ T cells, but is dispensable for sustaining their effector functions and their ability to induce disease. NOD mice (NOD/ShiLtJ) and 8.3 TCR transgenic NOD mice [NOD.Cg-Tg(TcraTcrbNY8.3)1Pesa/DvsJ; for brevity, 8.3-NOD] were purchased from the Jackson Laboratory (Bar Harbor, ME, USA). Il21−/− mice generated in a 129/SvEvBrd × C57Bl/6/J background (Lexicon Genetics Inc., The Woodlands, TX, USA) were obtained from MMRRC (Mutant Mouse Regional Resource Centre, Jackson Laboratory), back-crossed to NOD mice for 10 generations and back-crossed further to 8.3-NOD mice for two generations. At the fifth back-cross, mice were genotyped for known Idd loci and were selected for further breeding. The progeny of the 11th back-cross were intercrossed to generate NOD.Il21−/−, NOD.Il21+/− and NOD.Il21+/+ littermates. Mice were housed in micro-isolated sterile cages under specific pathogen-free (SPF) conditions. All experimental protocols were approved by the institutional ethical committee. Antibodies against mouse CD3ε, CD4, CD8α, TCRVβ8.

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