AggFluor: Fluorogenic Toolbox Enables Direct Visualization of the Multi-Step Protein Aggregation Process in Live Cells

化学 生物物理学 蛋白质聚集 活体细胞成像 荧光 发色团 纳米技术 费斯特共振能量转移 细胞 生物化学 光化学 量子力学 生物 物理 材料科学
作者
Charles H. Wolstenholme,Hang Hu,Songtao Ye,Brian E. Funk,Divya Jain,Chia-Heng Hsiung,Gang Ning,Yu Liu,Xiaosong Li,Xin Zhang
出处
期刊:Journal of the American Chemical Society [American Chemical Society]
卷期号:142 (41): 17515-17523 被引量:101
标识
DOI:10.1021/jacs.0c07245
摘要

Aberrantly processed or mutant proteins misfold and assemble into a variety of soluble oligomers and insoluble aggregates, a process that is associated with an increasing number of diseases that are not curable or manageable. Herein, we present a chemical toolbox, AggFluor, that allows for live cell imaging and differentiation of complex aggregated conformations in live cells. Based on the chromophore core of green fluorescent proteins, AggFluor is comprised of a series of molecular rotor fluorophores that span a wide range of viscosity sensitivity. As a result, these compounds exhibit differential turn-on fluorescence when incorporated in either soluble oligomers or insoluble aggregates. This feature allows us to develop, for the first time, a dual-color imaging strategy to distinguish unfolded protein oligomers from insoluble aggregates in live cells. Furthermore, we have demonstrated how small molecule proteostasis regulators can drive formation and disassembly of protein aggregates in both conformational states. In summary, AggFluor is the first set of rationally designed molecular rotor fluorophores that evenly cover a wide range of viscosity sensitivities. This set of fluorescent probes not only change the status quo of current imaging methods to visualize protein aggregation in live cells but also can be generally applied to study other biological processes that involve local viscosity changes with temporal and spatial resolutions.
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