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Quantitative Assay of Recombinant Hepatitis B Surface Antigen by Using Surface Plasmon Resonance Biosensor  

Lee, E. K. (Department of Chemical Engineering Bioprocessing Research Laboratory Hanyang University Ansan)
Ahn, S. J. (Department of Biochemistry and Molecular Biology, Hanyang University Ansan)
Yoo, C. H. (Department of Chemical Engineering Bioprocessing Research Laboratory Hanyang University Ansan)
Ryu, K. (Department of Chemical Engineering Bioprocessing Research Laboratory Hanyang University Ansan)
Jeon, J. Y. (DI Biotech, Ltd.)
Lee, H. I. (DI Biotech, Ltd.)
Choi, S. C. (Greencross Vaccine Corp., GE Team Yongin)
Lee, Y. S. (Department of Chemical Engineering Bioprocessing Research Laboratory Hanyang University Ansan)
Publication Information
KSBB Journal / v.17, no.1, 2002 , pp. 20-25 More about this Journal
Abstract
We performed a basic experiment for rapid, on-line, real-time measurement of HBsAg by using a surface plasmon resonance biosensor to quantify the recognition and interaction of biomolecules. We immobilized the anti-HBsAg polyclonal antibody to the dextran layer on a CM5 chip surface which was pre-activated by N-hydroxysuccinimide for amine coupling. The binding of the HBsAg to the immobilized antibody was measured by the mass increase detected by the change in the SPR signal. The binding characteristics between HBsAg and its antibody followed typical monolayer adsorption isotherm. When the entire immobilized antibody was interacted, there was no additional, non-specific binding observed, which suggested the biointeraction was very specific as expected and independent of the ligand density. No significant steric hindrance was observed at 17.6 nm/$mm^2$ immobilization density. The relationship between the HBsAg concentration in the sample solution and the antigen bound to the chip surface was linear up to ca. $40\mu\textrm{g}$/mL, which is much wider than that of the ELISA method. It appeared the antigen-antibody binding was increased as the immobilized ligand density increased, but verification is warranted. This study showed the potential of this biosensor-based method as a rapid, simple, multi-sample, on-line assay. Once properly validated, it can serve as a more powerful method for HBsAg quantification replacing the current ELISA method.
Keywords
biosensor; HBsAg; virus assay; SPR;
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