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胺基修饰以最大化蛋白-染料荧光和超稳定蛋白-配体相互作用。

Amine Landscaping to Maximize Protein-Dye Fluorescence and Ultrastable Protein-Ligand Interaction.

机构信息

Department of Biochemistry, University of Oxford, South Parks Road, Oxford OX1 3QU, UK.

Wallenberg Laboratory, Department of Molecular and Clinical Medicine, Institute of Medicine, University of Gothenburg, Gothenburg, Sweden.

出版信息

Cell Chem Biol. 2017 Aug 17;24(8):1040-1047.e4. doi: 10.1016/j.chembiol.2017.06.015. Epub 2017 Jul 27.

Abstract

Chemical modification of proteins provides great opportunities to control and visualize living systems. The most common way to modify proteins is reaction of their abundant amines with N-hydroxysuccinimide (NHS) esters. Here we explore the impact of amine number and positioning on protein-conjugate behavior using streptavidin-biotin, a central research tool. Dye-NHS modification of streptavidin severely damaged ligand binding, necessitating development of a new streptavidin-retaining ultrastable binding after labeling. Exploring the ideal level of dye modification, we engineered a panel bearing 1-6 amines per subunit: "amine landscaping." Surprisingly, brightness increased as amine number decreased, revealing extensive quenching following conventional labeling. We ultimately selected Flavidin (fluorophore-friendly streptavidin), combining ultrastable ligand binding with increased brightness after conjugation. Flavidin enhanced fluorescent imaging, allowing more sensitive and specific cell labeling in tissues. Flavidin should have wide application in molecular detection, providing a general insight into how to optimize simultaneously the behavior of the biomolecule and the chemical probe.

摘要

蛋白质的化学修饰为控制和可视化生命系统提供了极好的机会。修饰蛋白质最常见的方法是将其丰富的胺与 N-羟基琥珀酰亚胺(NHS)酯反应。在这里,我们使用链霉亲和素-生物素研究了胺数量和位置对蛋白质缀合物行为的影响,链霉亲和素-生物素是一种重要的研究工具。染料-NHS 修饰的链霉亲和素严重破坏了配体结合,因此需要在标记后开发一种新的保持链霉亲和素的超稳定结合。为了探索理想的染料修饰水平,我们设计了一组每个亚基带有 1-6 个胺的面板:“胺地形”。令人惊讶的是,随着胺数量的减少,亮度增加,表明在传统标记后存在广泛的猝灭。我们最终选择了 Flavidin(荧光染料友好型链霉亲和素),它在结合后具有超稳定的配体结合和增加的亮度。Flavidin 增强了荧光成像,使组织中的细胞标记更加敏感和特异。Flavidin 应该在分子检测中有广泛的应用,为如何同时优化生物分子和化学探针的行为提供了一般性的见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/46e9/5563079/523012e069d2/fx1.jpg

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