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开发一种用于测量化合物结合动力学的细胞内定量测定法。

Development of an intracellular quantitative assay to measure compound binding kinetics.

机构信息

Division of Physiology, Pharmacology and Neuroscience, School of Life Sciences, University of Nottingham, Nottingham NG7 2UH, UK; Medicine Design, Medicinal Science and Technology, GlaxoSmithKline, Stevenage SG1 2NY, UK.

Medicine Design, Medicinal Science and Technology, GlaxoSmithKline, Stevenage SG1 2NY, UK; Arctoris, Oxford OX14 4SA, UK.

出版信息

Cell Chem Biol. 2022 Feb 17;29(2):287-299.e8. doi: 10.1016/j.chembiol.2021.07.018. Epub 2021 Sep 13.

Abstract

Contemporary drug discovery typically quantifies the effect of a molecule on a biological target using the equilibrium-derived measurements of IC, EC, or K. Kinetic descriptors of drug binding are frequently linked with the effectiveness of a molecule in modulating a disease phenotype; however, these parameters are yet to be fully adopted in early drug discovery. Nanoluciferase bioluminescence resonance energy transfer (NanoBRET) can be used to measure interactions between fluorophore-conjugated probes and luciferase fused target proteins. Here, we describe an intracellular NanoBRET competition assay that can be used to quantify cellular kinetic rates of compound binding to nanoluciferase-fused bromodomain and extra-terminal (BET) proteins. Comparative rates are generated using a cell-free NanoBRET assay and by utilizing orthogonal recombinant protein-based methodologies. A screen of known pan-BET inhibitors is used to demonstrate the value of this approach in the investigation of kinetic selectivity between closely related proteins.

摘要

当代药物发现通常使用 IC、EC 或 K 的平衡衍生测量来量化分子对生物靶标的作用。药物结合的动力学描述符通常与分子调节疾病表型的有效性相关联;然而,这些参数尚未在早期药物发现中得到充分采用。纳米荧光素酶生物发光共振能量转移(NanoBRET)可用于测量荧光探针缀合物与荧光素酶融合靶蛋白之间的相互作用。在这里,我们描述了一种细胞内 NanoBRET 竞争测定法,可用于定量化合物与纳米荧光素酶融合溴结构域和额外末端(BET)蛋白结合的细胞内动力学速率。使用无细胞 NanoBRET 测定法和利用正交重组蛋白基方法学生成比较速率。对已知的泛 BET 抑制剂进行筛选,以证明该方法在研究密切相关的蛋白质之间的动力学选择性方面的价值。

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