Figure 4.
Figure 4. Characterization of FBG-325 and FBG-ΔAαC. FBG-325 was analyzed by SDS-PAGE under nonreducing (A) and reducing (B) conditions followed by Coomassie blue staining. The positions of migration of intact FBG (340 kDa), FBG-325 (325 kDa), and reduced FBG Aα, Bβ, BβΔ1-42, and γ chains are marked. ELISA (C) was performed using serial dilutions of MoAb 18C6 to detect the presence (FBG, □) or absence (FBG-325, •) of Bβ1-21. Western blot analysis using MoAbs against FPA, Aα87-100 containing the RGDF95-98 domain, and Aα566-580 containing the RGDS572-575 domain was performed on FBG and FBG-ΔAαC resolved under nonreducing (D) or reducing (E) conditions.

Characterization of FBG-325 and FBG-ΔAαC. FBG-325 was analyzed by SDS-PAGE under nonreducing (A) and reducing (B) conditions followed by Coomassie blue staining. The positions of migration of intact FBG (340 kDa), FBG-325 (325 kDa), and reduced FBG Aα, Bβ, BβΔ1-42 , and γ chains are marked. ELISA (C) was performed using serial dilutions of MoAb 18C6 to detect the presence (FBG, □) or absence (FBG-325, •) of Bβ1-21 . Western blot analysis using MoAbs against FPA, Aα87-100 containing the RGDF95-98 domain, and Aα566-580 containing the RGDS572-575 domain was performed on FBG and FBG-ΔAαC resolved under nonreducing (D) or reducing (E) conditions.

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