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Measurement of Small Molecule Binding Kinetics ona Protein Microarray by Plasmonic-Based Electrochemical ImpedanceImaging

机译:小分子结合动力学的测量。通过基于等离子体的电化学阻抗的蛋白质芯片影像学

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摘要

We report on a quantitative study of small molecule binding kinetics on protein microarrays with plasmonic-based electrochemical impedance microscopy (P-EIM). P-EIM measures electrical impedance optically with high spatial resolution by converting a surface charge change to a surface plasmon resonance (SPR) image intensity change, and the signal is not scaled to the mass of the analyte. Using P-EIM, we measured binding kinetics and affinity between small molecule drugs (imatinib and SB202190) and their target proteins (kinases Abl1 and p38-α). The measured affinity values are consistent with reported values measured by an indirect competitive binding assay. We also found that SB202190 has weak bindings to ABL1 with KD > 10 μM, which is not reported in the literature. Furthermore, we found that P-EIM is less prone to nonspecific binding, a long-standing issue in SPR. Our results show that P-EIM is a novel method for high-throughput measurement of small molecule binding kinetics and affinity, whichis critical to the understanding of small molecules in biologicalsystems and discovery of small molecule drugs.
机译:我们报告了基于等离激元的电化学阻抗显微镜(P-EIM)的蛋白质微阵列上的小分子结合动力学的定量研究。 P-EIM通过将表面电荷变化转换为表面等离振子共振(SPR)图像强度变化,从而以高空间分辨率光学测量电阻抗,并且信号未按比例缩放到分析物的质量。使用P-EIM,我们测量了小分子药物(伊马替尼和SB202190)与其靶蛋白(激酶Abl1和p38-α)之间的结合动力学和亲和力。测得的亲和力值与通过间接竞争结合测定法测得的报道值一致。我们还发现SB202190与KBL> 10μM的ABL1结合较弱,这在文献中未见报道。此外,我们发现P-EIM不易发生非特异性结合,这是SPR中长期存在的问题。我们的结果表明,P-EIM是一种用于小分子结合动力学和亲和力的高通量测量的新方法,对于了解生物中的小分子至关重要系统和小分子药物的发现。

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