Unlocking latent kinetic information from label-free binding

被引:3
|
作者
Quinn, John G. [1 ]
Steffek, Micah [1 ]
Bruning, John M. [1 ]
Frommlet, Alexandra [1 ]
Mulvihill, Melinda M. [1 ]
机构
[1] Genentech Inc, Biochem & Cellular Pharmacol, Biophys Grp, 1 DNA Way, San Francisco, CA 94080 USA
关键词
DIFFUSION; CONVECTION; CONSTANTS; MECHANISM; BIACORE;
D O I
10.1038/s41598-019-54485-4
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
Transient affinity binding interactions are central to life, composing the fundamental elements of biological networks including cell signaling, cell metabolism and gene regulation. Assigning a defined reaction mechanism to affinity binding interactions is critical to our understanding of the associated structure-function relationship, a cornerstone of biophysical characterization. Transient kinetics are currently measured using low throughput methods such as nuclear magnetic resonance, or stop-flow spectrometry-based techniques, which are not practical in many settings. In contrast, label-free biosensors measure reaction kinetics through direct binding, and with higher throughout, impacting life sciences with thousands of publications each year. Here we have developed a methodology enabling label-free biosensors to measure transient kinetic interactions towards providing a higher throughput approach suitable for mechanistic understanding of these processes. The methodology relies on hydrodynamic dispersion modeling of a smooth analyte gradient under conditions that maintain the quasi-steady-state boundary layer assumption. A transient peptide-protein interaction of relevance to drug discovery was analyzed thermodynamically using transition state theory and numerical simulations validated the approach over a wide range of operating conditions. The data establishes the technical feasibility of this approach to transient kinetic analyses supporting further development towards higher throughput applications in life science.
引用
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页数:9
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