Biosensors (Jan 2015)

Kinetic Analyses of Data from a Human Serum Albumin Assay Using the liSPR System

  • Anja Henseleit,
  • Carolin Pohl,
  • Hans-Michael Kaltenbach,
  • Karina Hettwer,
  • Kirsten Simon,
  • Steffen Uhlig,
  • Natalie Haustein,
  • Thomas Bley,
  • Elke Boschke

DOI
https://doi.org/10.3390/bios5010027
Journal volume & issue
Vol. 5, no. 1
pp. 27 – 36

Abstract

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We used the interaction between human serum albumin (HSA) and a high-affinity antibody to evaluate binding affinity measurements by the bench-top liSPR system (capitalis technology GmbH). HSA was immobilized directly onto a carboxylated sensor layer, and the mechanism of interaction between the antibody and HSA was investigated. The bivalence and heterogeneity of the antibody caused a complex binding mechanism. Three different interaction models (1:1 binding, heterogeneous analyte, bivalent analyte) were compared, and the bivalent analyte model best fit the curves obtained from the assay. This model describes the interaction of a bivalent analyte with one or two ligands (A + L ↔ LA + L ↔ LLA). The apparent binding affinity for this model measured 37 pM for the first reaction step, and 20 pM for the second step.

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