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Determination of Rate Constants and Equilibrium Constants for Solution-Phase Drug-Protein Interactions by Ultrafast Affinity Extraction

机译:超快速亲和萃取法测定溶液相药物-蛋白质相互作用的速率常数和平衡常数

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A method was created on the basis of ultrafast affinity extraction to determine both the dissociation rate constants and equilibrium constants for drug--protein interactions in solution. Human serum albumin (HSA), an important binding agent for many drugs in blood, was used as both a model soluble protein and as an immobilized binding agent in affinity microcolumns for the analysis of free drug fractions. Several drugs were examined that are known to bind to HSA. Various conditions to optimize in the use of ultrafast affinity extraction for equilibrium and kinetic studies were considered, and several approaches for these measurements were examined. The dissociation rate constants obtained for soluble HSA with each drug gave good agreement with previous rate constants reported for the same drugs or other solutes with comparable affinities for HSA. The equilibrium constants that were determined also showed good agreement with the literature. The results demonstrated that ultrafast affinity extraction could be used as a rapid approach to provide information on both the kinetics and thermodynamics of a drug--protein interaction in solution. This approach could be extended to other systems and should be valuable for high-throughput drug screening or biointeraction studies.
机译:在超快亲和萃取的基础上创建了一种方法,以确定溶液中药物-蛋白质相互作用的解离速率常数和平衡常数。人血清白蛋白(HSA)是血液中许多药物的重要结合剂,既用作模型可溶性蛋白,又用作亲和微柱中的固定结合剂,用于分析游离药物组分。检查了几种已知与HSA结合的药物。考虑了在使用超快亲和萃取进行平衡和动力学研究中优化的各种条件,并研究了这些测量的几种方法。可溶性HSA与每种药物的解离速率常数与先前报道的相同药物或对HSA具有相似亲和力的其他溶质的速率常数非常吻合。确定的平衡常数也与文献显示出良好的一致性。结果表明,超快亲和萃取可以用作提供有关溶液中药物-蛋白质相互作用的动力学和热力学信息的快速方法。这种方法可以扩展到其他系统,并且对高通量药物筛选或生物相互作用研究具有参考价值。

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