APC-protamine anticoagulant synergy is not mediated by enhanced substrate proteolysis. (A) FVa proteolysis by APC was assessed in both the absence (▲) and presence (○) of 3 μg/mL protamine. Purified FVa (1 nM final concentration) was incubated with phospholipid vesicles (PC:PS:PE, 60%:20%:20%, 20 μM final concentration) in a buffer containing 175 mM NaCl, 3 mM CaCl2, and 25 mM HEPES (pH 7.4) at 37°C. APC (2 nM final concentration) was added to initiate FVa inactivation. At specific time points, aliquots of the reaction mix were added to a separate prothrombinase mixture and thrombin generated was measured, as described in “Methods.” (B) To assess FVIIIa proteolysis by APC, thrombin generation was initiated with TF, phospholipid vesicles, and CaCl2 in FVIII-deficient plasma to which 1.0 U/mL wild-type (□) or APC-resistant FVIII R336Q/R562Q (■), respectively, had been added. ETP was determined for each FVIII variant in the presence and absence of protamine (3 μg/mL) and also in the presence of APC (10 nM).