Arylamino-substituted Rhodamine as a Fluorogenic Molecular Rotor for the Wash-free Imaging of Non-catalytic Proteins in Live Cells

IF 3.4 Q2 CHEMISTRY, ANALYTICAL
Huiling Tang, Xia Yuan, Yefeng Chen, Dr. Yuyao Li, Prof. Dr. Xiaoyong Xu, Prof. Dr. Hexin Xie
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引用次数: 0

Abstract

Fluorescent probes are valuable tools to visualize non-catalytic proteins in live cells. Currently, the majority of imaging reagents for non-catalytic proteins are based on “always-on” fluorophores and the use of these reagents usually necessitate a wash step to remove unbounded fluorophores before microscope imaging. Herein, we report the use of arylamino-substituted rhodamine as an activatable fluorophore for the imaging of non-catalytic protein in live cells. We have shown the induction of an arylamino to structurally rigid rhodamine could significantly reduce the fluorescent emission in aqueous medium but the ligand-directed binding of this molecule to protein receptor could effective restrict its intramolecular motion and thus lead to enhancement in fluorescence intensity at 590 nm over 30-fold. With fluorescent probes based on this fluorophore, we could visualize integrin αvβ3 and azido-functionalized glycans in living cells with high contrast in a wash-free manner.

Abstract Image

芳基氨基取代的罗丹明作为荧光分子旋转剂,用于活细胞中非催化蛋白质的免洗成像
荧光探针是观察活细胞中非催化蛋白质的重要工具。目前,大多数用于非催化蛋白质的成像试剂都是基于 "始终开启 "的荧光团,使用这些试剂通常需要在显微镜成像前进行清洗步骤以去除未结合的荧光团。在此,我们报告了使用芳基氨基取代的罗丹明作为可激活的荧光团,对活细胞中的非催化蛋白质进行成像。我们的研究表明,将芳基氨基诱导到结构刚性的罗丹明中可显著降低其在水介质中的荧光发射,但该分子与蛋白质受体的配体定向结合可有效限制其分子内运动,从而使其在 590 纳米波长处的荧光强度增强 30 倍以上。利用基于这种荧光探针的荧光探针,我们可以在活细胞中以高对比度、免清洗的方式观察整合素 αvβ3 和叠氮功能化聚糖。
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CiteScore
2.60
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