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Parallelized Ligand Screening Using Dissolution Dynamic Nuclear Polarization.利用溶解动态核极化进行并行配体筛选。
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Milli-tesla NMR and spectrophotometry of liquids hyperpolarized by dissolution dynamic nuclear polarization.通过溶解动态核极化实现液体超极化后的毫特斯拉核磁共振和分光光度法。
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Site specific polarization transfer from a hyperpolarized ligand of dihydrofolate reductase.来自二氢叶酸还原酶超极化配体的位点特异性极化转移。
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Hyperpolarized Water to Study Protein-Ligand Interactions.用于研究蛋白质-配体相互作用的超极化水
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溶解动态核极化技术在核磁共振筛选中的应用。

Applications of Dissolution-DNP for NMR Screening.

作者信息

Kim Yaewon, Hilty Christian

机构信息

Chemistry Department, Texas A&M University, College Station, TX, United States.

Chemistry Department, Texas A&M University, College Station, TX, United States.

出版信息

Methods Enzymol. 2019;615:501-526. doi: 10.1016/bs.mie.2018.08.016. Epub 2018 Dec 4.

DOI:10.1016/bs.mie.2018.08.016
PMID:30638540
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8179729/
Abstract

Experimental screening for protein-ligand interactions is a central task in drug discovery. Nuclear magnetic resonance (NMR) spectroscopy enables the determination of binding affinities, as well as the measurement of structural and dynamic parameters governing the interaction. With traditional liquid-state NMR relying on a nuclear spin polarization on the order of 10, hyperpolarization methods such as dissolution dynamic nuclear polarization (D-DNP) can increase signals by several orders of magnitude. The resulting increase in sensitivity has the potential to reduce requirements for the concentration of protein and ligands, improve the accuracy of the detection of interaction by allowing the use of near-stoichiometric conditions, and increase throughput. This chapter introduces a selection of basic techniques for the application of D-DNP to screening. Procedures for hyperpolarization are briefly reviewed, followed by the description of NMR methods for detection of binding through changes in chemical shift and relaxation parameters. Experiments employing competitive binding with a known ligand are shown, which can be used to determine binding affinity or yield structural information on the pharmacophore. The specific challenges of working with nonrenewable hyperpolarization are reviewed, and solutions including the use of multiplexed NMR detection are described. Altogether, the methods summarized in this chapter are intended to allow for the efficient detection of binding affinity, structure, and dynamics facilitated through substantial signal enhancements provided by hyperpolarization.

摘要

蛋白质-配体相互作用的实验筛选是药物发现中的核心任务。核磁共振(NMR)光谱能够测定结合亲和力,以及测量控制相互作用的结构和动力学参数。传统的液态NMR依赖于约为10的核自旋极化,而诸如溶解动态核极化(D-DNP)等超极化方法可以将信号增强几个数量级。由此带来的灵敏度提高有可能降低对蛋白质和配体浓度的要求,通过允许使用接近化学计量比的条件来提高相互作用检测的准确性,并提高通量。本章介绍了一系列将D-DNP应用于筛选的基本技术。简要回顾了超极化的程序,随后描述了通过化学位移和弛豫参数变化检测结合的NMR方法。展示了采用与已知配体竞争性结合的实验,这些实验可用于确定结合亲和力或获得药效团的结构信息。综述了使用不可再生超极化时面临的具体挑战,并描述了包括使用多路复用NMR检测在内的解决方案。总之,本章总结的方法旨在通过超极化提供的大幅信号增强来实现对结合亲和力、结构和动力学的高效检测。