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A Multi-Step NMR Screen for the Identification and Evaluation of Chemical Leads for Drug Discovery

机译:用于鉴定和评估用于药物发现的化学铅的多步NMR筛选

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摘要

A multi-step NMR based screening assay is described for identifying and evaluating chemical leads for their ability to bind a target protein. The multi-step NMR assay provides structure-related information while being an integral part of a structure based drug discovery and design program. The fundamental principle of the multi-step NMR assay is to combine distinct 1D and 2D NMR techniques, in such a manner, that the inherent strengths and weakness associated with each technique is complementary to each other in the screen. By taking advantage of the combined strengths of 1D and 2D NMR experiments, it is possible to minimize protein requirements and experiment time and differentiate between nonspecific and stoichiometric binders while being able to verify ligand binding, determine a semi-quantitative dissociation constant, identify the ligand binding site and rapidly determine a protein-ligand co-structure. Furthermore, the quality and physical behavior of the ligand is readily evaluated to determine its appropriateness as a chemical lead. The utility of the multi-step NMR assay is demonstrated with the use of PrgI from Salmonella typhimurium and human serum albumin (HSA) as target proteins.
机译:描述了基于多步NMR的筛选测定法,用于鉴定和评估化学引线结合靶蛋白的能力。多步NMR分析可提供与结构相关的信息,同时也是基于结构的药物发现和设计程序的组成部分。多步NMR分析的基本原理是以这种方式结合不同的1D和2D NMR技术,使得与每种技术相关的固有优势和劣势在屏幕上彼此互补。通过利用1D和2D NMR实验的结合强度,可以最小化蛋白质需求和实验时间,并区分非特异性和化学计量的结合物,同时能够验证配体结合,确定半定量解离常数,鉴定配体结合位点并迅速确定蛋白质-配体的共结构。此外,容易评估配体的质量和物理行为,以确定其作为化学铅的适当性。通过使用鼠伤寒沙门氏菌的PrgI和人血清白蛋白(HSA)作为靶蛋白,证明了多步NMR测定的实用性。

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