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荧光核苷类似物在高通量抑制剂筛选中的应用。

Deploying Fluorescent Nucleoside Analogues for High-Throughput Inhibitor Screening.

机构信息

Department of Biology and Department of Chemistry, Massachusetts Institute of Technology, Cambridge, MA, 02139, USA.

出版信息

Chembiochem. 2020 Jan 15;21(1-2):108-112. doi: 10.1002/cbic.201900671. Epub 2019 Dec 3.

Abstract

High-throughput small-molecule screening in drug discovery processes commonly rely on fluorescence-based methods including fluorescent polarization and fluorescence/Förster resonance energy transfer. These techniques use highly accessible instrumentation; however, they can suffer from high false-negative rates and background signals, or might involve complex schemes for the introduction of fluorophore pairs. Herein we present the synthesis and application of fluorescent nucleoside analogues as the foundation for directed approaches for competitive binding analyses. The general approach describes selective fluorescent environment-sensitive (ES) nucleoside analogues that are adaptable to diverse enzymes that act on nucleoside-based substrates. We demonstrate screening a set of uridine analogues and development of an assay for fragment-based lead discovery with the TcdB glycosyltransferase (GT), an enzyme associated with virulence in Clostridium difficile. The uridine-based probe used for this high-throughput screen has a K value of 7.2 μm with the TcdB GT and shows a >30-fold increase in fluorescence intensity upon binding. The ES-based probe assay is benchmarked against two other screening approaches.

摘要

高通量小分子药物筛选在药物发现过程中通常依赖于荧光为基础的方法,包括荧光偏振和荧光/Förster 共振能量转移。这些技术使用了易于获得的仪器;然而,它们可能会受到高假阴性率和背景信号的影响,或者可能涉及引入荧光团对的复杂方案。在此,我们提出了荧光核苷类似物的合成和应用,作为竞争性结合分析的定向方法的基础。一般方法描述了选择性荧光环境敏感 (ES) 核苷类似物,这些类似物适用于作用于核苷底物的多种酶。我们展示了对一组尿苷类似物的筛选,并开发了一种用于片段基 Lead Discovery 的测定方法,用于 TcdB 糖基转移酶 (GT),该酶与艰难梭菌的毒力有关。用于这种高通量筛选的基于尿苷的探针与 TcdB GT 的 K 值为 7.2μm,并在结合时显示荧光强度增加超过 30 倍。ES 探针测定法与其他两种筛选方法进行了基准测试。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f7d1/6980326/5990164004bb/nihms-1064644-f0001.jpg

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