Effect of FXII-concentration on fibrin structure in plasma. (A) FXII-deficient plasma was reconstituted with purified FXII, and clotting was initiated via contact activation with sulfatides, in the presence of phospholipid vesicles and CaCl₂. Turbidity was monitored every 15 seconds at 405 nm at 37°C. Final concentrations were 76% plasma, variable FXII concentrations (0%-100% of normal plasma concentration), 4μM sulfatides, 4μM phospholipid vesicles, and 16mM CaCl₂. Data are mean ± range of 3 measurements. (B) Representative figures of immunofluorescent staining of fibrin clots. FXII-deficient plasma was reconstituted with purified FXII. Alexa Fluor–488 fibrinogen was added, and clotting was initiated with sulfatide, phospholipid vesicles, and CaCl₂. Final concentrations were 25% plasma, 5% Alexa Fluor–488 fibrinogen of the total fibrinogen concentration, a range of FXII (0%-100% of normal plasma concentration), 0.4μM sulfatides, 4μM phospholipid vesicles, 5mM CaCl₂, 25mM HEPES (pH 7.4), and 150mM NaCl. (C) Fiber density was calculated from the data shown in panel B. Per condition, 2 separate clots were made, images were taken in different areas of the clot, and fiber density was determined in 5 images by counting the number of fibers that cross a line of 100 μm. Bars represent mean ± SEM. *P < .05. Scale bars represent 25 μm.