Figure 6
Figure 6. The permeability barrier-enhancing effect of thrombin is reversed by the ligand occupancy of EPCR with PC-S195A, but not with factor VIIa. EA.hy926 cells were incubated with APC (10 nmol/L) and thrombin (2 nmol/L) in the absence and presence of either PC-S195A or factor VIIa (50 nmol/L) for 3 hours before inducing permeability with 5 nmol/L thrombin for 10 minutes. B-αEPCR is blocking anti-EPCR (clone RCR-252), B-αPAR-1 (H-111) is blocking anti-PAR-1, and NB-αPAR-1 (S-19) is nonblocking anti-PAR-1, which have been incubated with endothelial cells for 30 minutes before treatment with APC. Baseline represents the permeability of untreated control cells not stimulated with thrombin. Error bars represent SD.

The permeability barrier-enhancing effect of thrombin is reversed by the ligand occupancy of EPCR with PC-S195A, but not with factor VIIa. EA.hy926 cells were incubated with APC (10 nmol/L) and thrombin (2 nmol/L) in the absence and presence of either PC-S195A or factor VIIa (50 nmol/L) for 3 hours before inducing permeability with 5 nmol/L thrombin for 10 minutes. B-αEPCR is blocking anti-EPCR (clone RCR-252), B-αPAR-1 (H-111) is blocking anti-PAR-1, and NB-αPAR-1 (S-19) is nonblocking anti-PAR-1, which have been incubated with endothelial cells for 30 minutes before treatment with APC. Baseline represents the permeability of untreated control cells not stimulated with thrombin. Error bars represent SD.

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