Equilibrium binding of antithrombin and thrombin to EP compounds. (A) Relative protein fluorescence changes (Fobs/Fo) accompanying the stepwise addition of EP42675 (open symbols) or EP217609 (closed symbols) to 500nM antithrombin in I 0.05 sodium phosphate buffer (○, ●) or to 200nM antithrombin in I 0.15 HEPES plus Ca2+ buffer (▵, ▴) both at pH 7.4, 25°C, are plotted as a function of the molar ratio of EP compound to antithrombin. Solid lines indicate fits to the quadratic equilibrium binding equation from which the binding stoichiometry, the KD (fixed at 0.5nM for I 0.05 titrations) and the maximal fluorescence change were derived. (B) Relative changes in p-aminobenzamidine fluorescence (Fobs/Fo) accompanying the stepwise addition of EP42675 (○) or EP217609 (●) to 200nM thrombin plus 100μM p-aminobenzamidine are plotted as a function of the molar ratio of EP compound to thrombin. Titrations were fit by the quadratic equilibrium binding equation in which KD was fixed at a value of 0.1nM based on measurements of KI and the competitive effect of probe binding to obtain values for the binding stoichiometry and maximal fluorescence change.