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Enzyme-Mediated, Site-Specific Protein Coupling Strategies for Surface-Based Binding Assays

机译:酶介导,基于表面的结合测定的特异性特异性蛋白质偶极策略

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摘要

Covalent surface immobilization of proteins for binding assays is typically performed non-specifically via lysine residues. However, receptors that either have lysines near their binding pockets, or whose presence at the sensor surface is electrostatically disfavoured, can be hard to probe. To overcome these limitations and to improve the homogeneity of surface functionalization, we adapted and optimized three different enzymatic coupling strategies (4'-phosphopantetheinyl transferase, sortase A, and asparaginyl endopeptidase) for biolayer interferometry surface modification. All of these enzymes can be used to site-specifically and covalently ligate proteins of interest via short recognition sequences. The enzymes function under mild conditions and thus immobilization does not affect the receptors' functionality. We successfully employed this enzymatic surface functionalization approach to study the binding kinetics of two different receptor-ligand pairs.
机译:用于结合测定的蛋白质的共价表面固定化通常通过赖氨酸残基进行非特异性进行。 然而,具有靠近其装订袋附近的赖氨酸的受体,或者在传感器表面的存在是静电脱离的,可能是难以探测的。 为了克服这些限制并改善表面官能化的均匀性,我们适应并优化了三种不同的酶促偶联策略(4'-磷酸乙乙基转移酶,分子A和天冬酰胺烯基内肽酶,用于Biolayer干涉式表面改性。 所有这些酶都可用于通过短识别序列特异性地和共价地与感兴趣的蛋白质。 在温和条件下的酶活性,因此固定不影响受体的功能。 我们成功地研制了这种酶表面官能化方法来研究两种不同受体 - 配体对的结合动力学。

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