Effect of Zn2+ on binding of FXIIa to HRG monitored by SPR. Biotin-HRG was adsorbed onto a streptavidin-coated sensor chip to 50 RU. Increasing concentrations of FXIIa (0-256nM) were injected at a flow rate of 45 μL/min in the presence of 2mM ethylenediaminetetraacetic acid (A) or 12.5μM ZnCl2 (B). FXIIa concentrations are indicated adjacent to each tracing, with the exception of 0.5 and 0.25nM, which were omitted for clarity. FXIIa association to the chip surface was monitored for 8 minutes followed by injection of HBS to monitor dissociation. RU values were corrected for background and plotted versus time. (C) b-HRG (800 RU) was immobilized on a streptavidin chip, and 10nM FXIIa was injected in the presence of 0 to 20μM ZnCl2 for 200 seconds (a), followed by Zn2+-containing buffer lacking FXIIa for 600 seconds (b). Dissociation was then observed in buffer lacking Zn2+ for 400 seconds (c). The micromolar concentrations of ZnCl2 are noted on each tracing.