Figure 5
Figure 5. Ligand blotting of PS and FXa to TFPI. TFPI proteins were electrophoresed on 12% SDS-PAGE gel and transferred to a nitrocellulose membrane. The amount of each protein that was electrophoresed and blotted is labeled at the top. (A-B) Binding of PS to TFPI. PS was used to probe the membrane, and the bound PS was detected by an anti-PS polyclonal antibody as described in “Ligand and Western blotting.” (C-D) Binding of FXa to TFPI. After PS detection in panels A and B, the membranes were stripped with 0.1mM glycine, pH 2.2, and reprobed with FXa. The bound FXa was then detected using a goat anti-FX polyclonal antibody as described in “Ligand and Western blotting.” The positions of molecular weight markers are indicated on the left.

Ligand blotting of PS and FXa to TFPI. TFPI proteins were electrophoresed on 12% SDS-PAGE gel and transferred to a nitrocellulose membrane. The amount of each protein that was electrophoresed and blotted is labeled at the top. (A-B) Binding of PS to TFPI. PS was used to probe the membrane, and the bound PS was detected by an anti-PS polyclonal antibody as described in “Ligand and Western blotting.” (C-D) Binding of FXa to TFPI. After PS detection in panels A and B, the membranes were stripped with 0.1mM glycine, pH 2.2, and reprobed with FXa. The bound FXa was then detected using a goat anti-FX polyclonal antibody as described in “Ligand and Western blotting.” The positions of molecular weight markers are indicated on the left.

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