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荧光标记核糖体作为分析抗生素结合的工具。

Fluorescently labeled ribosomes as a tool for analyzing antibiotic binding.

作者信息

Llano-Sotelo Beatriz, Hickerson Robyn P, Lancaster Laura, Noller Harry F, Mankin Alexander S

机构信息

Center for Pharmaceutical Biotechnology, University of Illinois, Chicago, Illinois 60607, USA.

出版信息

RNA. 2009 Aug;15(8):1597-604. doi: 10.1261/rna.1681609. Epub 2009 Jun 24.

Abstract

Measuring the binding of antibiotics and other small-molecular-weight ligands to the 2.5 MDa ribosome often presents formidable challenges. Here, we describe a general method for studying binding of ligands to ribosomes that carry a site-specific fluorescent label covalently attached to one of the ribosomal proteins. As a proof of principle, an environment-sensitive fluorescent group was placed at several specific sites within the ribosomal protein S12. Small ribosomal subunits were reconstituted from native 16S rRNA, individually purified small subunit proteins, and fluorescently labeled S12. The fluorescence characteristics of the reconstituted subunits were affected by several antibiotics, including streptomycin and neomycin, which bind in the vicinity of protein S12. The equilibrium dissociation constants of the drugs obtained using a conventional fluorometer were in good agreement with those observed using previously published methods and with measurements based on the use of radiolabeled streptomycin. The newly developed method is rapid and sensitive, and can be used for determining thermodynamic and kinetic binding characteristics of antibiotics and other small ribosomal ligands. The method can readily be adapted for use in high-throughput screening assays.

摘要

测量抗生素及其他小分子配体与2.5兆道尔顿核糖体的结合情况往往面临巨大挑战。在此,我们描述了一种研究配体与核糖体结合的通用方法,该核糖体带有一个与核糖体蛋白之一共价连接的位点特异性荧光标记。作为原理验证,在核糖体蛋白S12内的几个特定位点放置了一个对环境敏感的荧光基团。从小牛16S rRNA、单独纯化的小亚基蛋白以及荧光标记的S12重构小核糖体亚基。重构亚基的荧光特性受到几种抗生素的影响,包括链霉素和新霉素,它们在蛋白S12附近结合。使用传统荧光计获得的药物平衡解离常数与使用先前发表的方法观察到的结果以及基于使用放射性标记链霉素的测量结果高度一致。新开发的方法快速且灵敏,可用于确定抗生素及其他小核糖体配体的热力学和动力学结合特性。该方法可轻松适用于高通量筛选测定。

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