Recombinant Mouse Antibody (AP33) is capable of binding to HCV E2 , expressed in Chinese Hamster Ovary cells (CHO). This mouse monoclonal antibody recognizes a conserved, linear epitope on E2 and potently neutralizes a broad range of HCV genotypes.
Figure 1 Inhibition of HCV-LPs binding to cells by anti-E1 and anti-E2 antibodies.
SYTO-labeled HCV-LPs were pre-incubated with 20 to 100μg of anti-E2 (AP33) for 2h at 4°C. The HCV-LP-antibody mixtures were then incubated with Molt-4 cells for 1 h. Flow cytometry histogram of HCV-LPs binding inthe presence (20 μg/ml) (open graph) or absence (black graph) of antibodies. The background binding is shown as the gray graph.
Triyatni, M., Saunier, B., Maruvada, P., Davis, A. R., Ulianich, L., Heller, T., ... & Liang, T. J. (2002). Interaction of hepatitis C virus-like particles and cells: a model system for studying viral binding and entry. Journal of virology, 76(18), 9335-9344.
Figure 2 Neutralization of HCVpp of genotype 1a using AP33 and e509 combinations.
Increasing concentrations of AP33 alone and in combination with e509 mAb at a fixed saturating concentration (10 μg/mL). The concentration of each mAb, alone or in combination, is reported on x axis. The neutralizing activity (y axis) is expressed as percent reduction infectivity of HCVpp of genotype 1a (H77 strain) without mAbs.
Sautto, G., Mancini, N., Diotti, R. A., Solforosi, L., Clementi, M., & Burioni, R. (2012). Anti-hepatitis C virus E2 (HCV/E2) glycoprotein monoclonal antibodies and neutralization interference. Antiviral research, 96(1), 82-89.
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(Creative Biolabs Cat# PABL-496, RRID: AB_3111660)
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