Adenosine A_2A receptor stimulation does not directly impair Tc1 or Tc2 cell cytolytic capacity. (A) Heteroconjugate assay reflective of granule exocytosis mediated cytolysis. ⁵¹Cr lysis assay was performed by incubating effector Tc1 and Tc2 cells (day 6 of culture) with P815 target cells in calcium replete media, with effector and target cell recognition mediated by anti-CD3 antibody (clone 2C11). Experimental groups included CGS (10^-8 and 10^-6 M; ▴ and ×, respectively); the control effector group was evaluated in DMSO vehicle (▪). An additional control group did not receive anti-CD3 (♦). E/T ratio indicates effector-target ratio. (B) Cytolysis via fas ligand. Fas ligand on Tc1 and Tc2 cells was induced with PMA and calcium ionophore, and cells were evaluated in ⁵¹Cr assays using wild-type (L1210) or fas-transfected (L1210-fas) targets in Ca⁺⁺-neutralized conditions. Tc1 and Tc2 effectors were incubated with CGS (10^-8 and 10^-6 M; ▴ and ×, respectively), or with vehicle control (DMSO; ▪); an additional control consisted of DMSO-treated Tc1 and Tc2 effectors and the nontransfected L1210 cell line as target (♦).