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Chromatographic study of the adsorption kinetics of albumin on monoclonal and polyclonal immunoadsorbents
Authors:C Vidal-Madjar  A Jaulmes  J Renard  D Peter  P Lafaye
Institution:(1) Laboratorie de Physico-Chimie des Biopolymères, CNRS, U.M.R. 27-Université Paris XII, 2 rue Henry Dunant, 94320 Thiais, France;(2) Hybridolab, Institut Pasteur, 75724 Paris Cedex 15, France
Abstract:Summary High-performance liquid chromatography (HPLC) has been used to study the adsorption kinetics of proteins on immunoadsorbents. The adsorption rate constant of human serum albumin (HSA) on monoclonal and polyclonal anti-HSA antibodies immobilized on a silica HPLC support was determined by saturating the column with repeated pulse injections. Studies on polyclonal immunodsorbents of different capacities enable evaluation of the contribution of transport to the binding sites. The adsorption properties of two different monoclonal anti-HSA antibodies immobilized on a chromatographic support were characterized by different approaches. The location of the epitope on the HSA molecule was determined by enzyme-linked immunoassay (ELISA) with albumin fragments. The chromatographic method was used to determine the column capacity and the adsorption rate constant of HSA on the immunoadsorbent. To compare the affinity of the antibodies for the antigen, an indirect ELISA method was used to determine the equilibrium constant of antigen-antibody association in solution Presented at the 21st ISC held in Stuttgart, Germany, 15th–20th september, 1996.
Keywords:Immunoaffinity chromatography  Adsorption kinetics  Human serum albumin  Monoclonal antibody
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