Figure 1
Figure 1. Absence of the TF allosteric disulfide results in abolished coagulant function. (A) BHK cells were stably transfected to express TFWT or TFCys209Ala. TF cell surface exposure was determined by labeling with 1mM NHS-biotin in HBS, and subsequently precipitation of biotinylated TF. To obtain total TF protein, immunoprecipitation with the TF mAb 9C3 was performed with n-octyl β-D-glucopyranoside (OG) cell lysates. Western Blotting was performed using Goat anti-TF antibody. The arrow indicates TF dimers. (B) Reactivity of a polyclonal goat anti-TF and 5G9 (both 10 μg/mL) with BHK cell surface levels of TFWT or TFCys209Ala. (C) TF procoagulant activity on nontransfected BHK cells, BHK-TFWT and BHK-TFCys209Ala was measured kinetically after addition of the indicated concentrations of VIIa and 100nM FX. (D) BHK cells expressing TFWT, TFCys209Ser and TFCys186/209Ser. Cell surface expression was determined after NHS-biotin labeling and total TF expression was determined in total lysate. Note the absence of a dimer fraction in case of the TFCys186/209Ser mutant. The arrow indicates TF dimers. (E) TF procoagulant activity on nontransfected BHK cells, BHK-TFWT, BHK-TFCys209Ser and BHK-TFCys186/209Ser was determined as described before. (F) BHK-TFWT and BHK-TFCys209Ser were incubated with 10mM N-ethylmaleimide for 1 hour. Presence of dimer factions was determined on Western blot and procoagulant activity was performed as described before, using 1nM VIIa.

Absence of the TF allosteric disulfide results in abolished coagulant function. (A) BHK cells were stably transfected to express TFWT or TFCys209Ala. TF cell surface exposure was determined by labeling with 1mM NHS-biotin in HBS, and subsequently precipitation of biotinylated TF. To obtain total TF protein, immunoprecipitation with the TF mAb 9C3 was performed with n-octyl β-D-glucopyranoside (OG) cell lysates. Western Blotting was performed using Goat anti-TF antibody. The arrow indicates TF dimers. (B) Reactivity of a polyclonal goat anti-TF and 5G9 (both 10 μg/mL) with BHK cell surface levels of TFWT or TFCys209Ala. (C) TF procoagulant activity on nontransfected BHK cells, BHK-TFWT and BHK-TFCys209Ala was measured kinetically after addition of the indicated concentrations of VIIa and 100nM FX. (D) BHK cells expressing TFWT, TFCys209Ser and TFCys186/209Ser. Cell surface expression was determined after NHS-biotin labeling and total TF expression was determined in total lysate. Note the absence of a dimer fraction in case of the TFCys186/209Ser mutant. The arrow indicates TF dimers. (E) TF procoagulant activity on nontransfected BHK cells, BHK-TFWT, BHK-TFCys209Ser and BHK-TFCys186/209Ser was determined as described before. (F) BHK-TFWT and BHK-TFCys209Ser were incubated with 10mM N-ethylmaleimide for 1 hour. Presence of dimer factions was determined on Western blot and procoagulant activity was performed as described before, using 1nM VIIa.

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