DOK1 and DOK2 regulate CD8 T cell signaling and memory formation without affecting tumor cell killing

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Laletin, Vladimir | Bernard, Pierre-Louis | Montersino, Camille | Yamamoto, Yuji, Y. | Olive, Daniel | Castellano, Rémy | Guittard, Geoffrey | Nunès, Jacques

Edité par CCSD ; Nature Publishing Group -

International audience. Abstract Targeting intracellular inhibiting proteins has been revealed to be a promising strategy to improve CD8 + T cell anti-tumor efficacy. Here, we are focusing on intracellular inhibiting proteins specific to TCR signaling: DOK1 and DOK2 expressed in T cells. We hypothesized that depletion of intracellular inhibition checkpoint DOK1 and DOK2 could improve CD8 + T-cell based cancer therapies. To evaluate the role of DOK1 and DOK2 depletion in physiology and effector function of CD8 + T lymphocytes and in cancer progression, we established a transgenic T cell receptor mouse model specific to melanoma antigen hgp100 (pmel-1 TCR Tg) in WT and Dok1 / Dok2 DKO (double KO) mice. We showed that both DOK1 and DOK2 depletion in CD8 + T cells after an in vitro pre-stimulation induced a higher percentage of effector memory T cells as well as an up regulation of TCR signaling cascade- induced by CD3 mAbs, including the increased levels of pAKT and pERK, two major phosphoproteins involved in T cell functions. Interestingly, this improved TCR signaling was not observed in naïve CD8 + T cells. Despite this enhanced TCR signaling essentially shown upon stimulation via CD3 mAbs, pre-stimulated Dok1 / Dok2 DKO CD8 + T cells did not show any increase in their activation or cytotoxic capacities against melanoma cell line expressing hgp100 in vitro. Altogether we demonstrate here a novel aspect of the negative regulation by DOK1 and DOK2 proteins in CD8 + T cells. Indeed, our results allow us to conclude that DOK1 and DOK2 have an inhibitory role following long term T cell stimulations.

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