PolyP and fibrin augment αFXIIa-mediated plasminogen activation. (A) Plasminogen activation was analyzed by incubating 200 nM αFXIIa and 200 nM Glu-plasminogen (dotted line) in the presence of either 3.8 μM soluble fibrin (SF; light gray), 70 μM polyP₇₀ (dark gray), or both SF and polyP₇₀ (black). Plasmin activity was detected using the chromogenic substrate S2251 at 405 nm. Data represent mean ± SEM (n = 3; P < .001). (B-C) The plasminogen activator function of αFXIIa (200 nM) was analyzed in the presence of different surfaces, including polyP₇₀ (70 μM), RNA (10 μg/mL), and collagen (5 μg/mL). (B) Plasmin activity, generated from 200 nM plasminogen, was detected using S2251. (C) Fibrinolysis was analyzed by forming clots from fibrinogen (3.8 μM), αFXIIa (200 nM), Glu-plasminogen (200 nM), thrombin (0.25 U/mL), and CaCl₂ (10 mM). Lysis was monitored at 405 nm, and mean ± SEM are shown as the time from maximal absorbance of the clot to 50% lysis (n = 3; ***P < .001). (D) Fibrin clots were formed and monitored as described in panel C, with 70 μM polyP₇₀ (black), 1 pM tPA (gray), or both polyP₇₀ and tPA (dark gray). The clots formed with tPA (dashed line) and both tPA and polyP (light gray) were formed in the absence of αFXIIa. Mean data ± SEM are expressed as percentage turbidity (n = 4; P < .0001).