Quantitation of Affinity, Avidity, and Binding Kinetics of Protein Analytes with a Dynamically Switchable Biosurface

被引:53
作者
Knezevic, Jelena
Langer, Andreas
Hampel, Paul A.
Kaiser, Wolfgang
Strasser, Ralf
Rant, Ulrich [1 ]
机构
[1] Tech Univ Munich, Walter Schottky Inst, D-85748 Garching, Germany
关键词
HISTIDINE-TAGGED PROTEINS; ELECTROCHEMICAL BIOSENSORS; BIOMOLECULAR INTERACTIONS; DNA LAYERS; SURFACE; NTA; ARCHITECTURES; RECOGNITION; INTERFACES; MONOLAYERS;
D O I
10.1021/ja3061276
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
A label-free method for the analysis of interactions of proteins with surface-tethered ligands is introduced. Short DNA levers are electrically actuated on microelectrodes by ac potentials, and their switching dynamics are measured in real-time by fluorescence energy transfer. Binding of proteins to ligands attached to the top of the DNA levers is detected by time-resolved measurements of the levers' dynamic motion. We demonstrate the quantitation of binding kinetics (k(on), k(off) rate constants), dissociation constants (K-D in the pM regime), and the influence of competitive binders (EC50 values). Moreover, the "switchSENSE" method reveals avidity effects and allows discriminating between analytes with one or more binding sites. In a comparative study, interactions of six hexa-histidine-tagged proteins with tris-nitrilotriacetic acid (NTA(3)) ligands are quantitated. Their binding kinetics and affinities are found to vary over up to 2 orders of magnitude, evidencing that the proteins' individual chemical environments significantly influence the His(6)-NTA(3) interaction.
引用
收藏
页码:15225 / 15228
页数:4
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