Journal for ImmunoTherapy of Cancer (Oct 2019)

Adenosine mediates functional and metabolic suppression of peripheral and tumor-infiltrating CD8+ T cells

  • Beatris Mastelic-Gavillet,
  • Blanca Navarro Rodrigo,
  • Laure Décombaz,
  • Haiping Wang,
  • Giuseppe Ercolano,
  • Rita Ahmed,
  • Leyder Elena Lozano,
  • Angela Ianaro,
  • Laurent Derré,
  • Massimo Valerio,
  • Thomas Tawadros,
  • Patrice Jichlinski,
  • Tu Nguyen-Ngoc,
  • Daniel E. Speiser,
  • Grégory Verdeil,
  • Nicolas Gestermann,
  • Olivier Dormond,
  • Lana Kandalaft,
  • George Coukos,
  • Camilla Jandus,
  • Christine Ménétrier-Caux,
  • Christophe Caux,
  • Ping-Chih Ho,
  • Pedro Romero,
  • Alexandre Harari,
  • Selena Vigano

DOI
https://doi.org/10.1186/s40425-019-0719-5
Journal volume & issue
Vol. 7, no. 1
pp. 1 – 16

Abstract

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Abstract Background Several mechanisms are present in the tumor microenvironment (TME) to impair cytotoxic T cell responses potentially able to control tumor growth. Among these, the accumulation of adenosine (Ado) contributes to tumor progression and represents a promising immunotherapeutic target. Ado has been shown to impair T cell effector function, but the role and mechanisms employed by Ado/Ado receptors (AdoRs) in modulating human peripheral and tumor-infiltrating lymphocyte (TIL) function are still puzzling. Methods CD8+ T cell cytokine production following stimulation was quantified by intracellular staining and flow cytometry. The cytotoxic capacity of tumor infiltrating lymphocytes (TILs) was quantified by the chromium release assay following co-culture with autologous or anti-CD3-loaded tumor cell lines. The CD8+ T cell metabolic fitness was evaluated by the seahorse assay and by the quantification of 2-NBDG uptake and CD71/CD98 upregulation upon stimulation. The expression of AdoRs was assessed by RNA flow cytometry, a recently developed technology that we validated by semiquantitative RT-PCR (qRT-PCR), while the impact on T cell function was evaluated by the use of selective antagonists and agonists. The influence of Ado/AdoR on the PKA and mTOR pathways was evaluated by phosphoflow staining of p-CREB and p-S6, respectively, and validated by western blot. Results Here, we demonstrate that Ado signaling through the A2A receptor (A2AR) in human peripheral CD8+ T cells and TILs is responsible for the higher sensitivity to Ado-mediated suppression of T central memory cells. We confirmed that Ado is able to impair peripheral and tumor-expanded T cell effector functions, and we show for the first time its impact on metabolic fitness. The Ado-mediated immunosuppressive effects are mediated by increased PKA activation that results in impairment of the mTORC1 pathway. Conclusions Our findings unveil A2AR/PKA/mTORC1 as the main Ado signaling pathway impairing the immune competence of peripheral T cells and TILs. Thus, p-CREB and p-S6 may represent useful pharmacodynamic and efficacy biomarkers of immunotherapies targeting Ado. The effect of Ado on T cell metabolic fitness reinforces the importance of the adenosinergic pathway as a target for next-generation immunotherapy.

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