P2Y 12 receptor blockade synergizes strongly with nitric oxide and prostacyclin to inhibit platelet activation

Aims In vivo platelet function is a product of intrinsic platelet reactivity, modifiable by dual antiplatelet therapy (DAPT), and the extrinsic inhibitory endothelial mediators, nitric oxide (NO) and prostacyclin (PGI 2 ), that are powerfully potentiated by P2Y 12 receptor blockade. This implies that for individual patients endothelial mediator production is an important determinant of DAPT effectiveness. Here, we have investigated this idea using platelets taken from healthy volunteers treated with anti‐platelet drugs. Methods Three groups of male volunteers ( n  = 8) received either prasugrel (10 mg), aspirin (75 mg) or DAPT (prasugrel + aspirin) once daily for 7 days. Platelet reactivity in the presence of diethylammonium (Z)‐1‐(N,N‐diethylamino)diazen‐1‐ium‐1,2‐diolate (DEA/NONOate) and PGI 2 was studied before and following treatment. Results Ex vivo , PGI 2 and/or DEA/NONOate had little inhibitory effect on TRAP‐6‐induced platelet reactivity in control conditions. However, in the presence of DAPT, combination of DEA/NONOate + PGI 2 reduced platelet aggregation (74 ± 3% to 19 ± 6%, P  < 0.05). In vitro studies showed even partial (25%) P2Y 12 receptor blockade produced a significant (67 ± 2% to 39 ± 10%, P  < 0.05) inhibition when DEA/NONOate + PGI 2 was present. Conclusions We have demonstrated that PGI 2 and NO synergize with P2Y 12 receptor antagonists to produce powerful platelet inhibition. Furthermore, even with submaximal P2Y 12 blockade the presence of PGI 2 and NO greatly enhances platelet inhibition. Our findings highlight the importance of endothelial mediator in vivo modulation of P2Y 12 inhibition and introduces the concept of refining ex vivo platelet function testing by incorporating an assessment of endothelial function to predict thrombotic outcomes better and adjust therapy to prevent adverse outcomes in individual patients.