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Literature DB >> 29883112

Modulation of Fluorescent Protein Chromophores To Detect Protein Aggregation with Turn-On Fluorescence.

Yu Liu, Charles H Wolstenholme, Gregory C Carter, Hongbin Liu¹, Hang Hu¹, Leeann S Grainger, Kun Miao, Matthew Fares, Conner A Hoelzel, Hemant P Yennawar, Gang Ning, Manyu Du, Lu Bai, Xiaosong Li¹, Xin Zhang.

Abstract

We present a fluorogenic method to visualize misfolding and aggregation of a specific protein-of-interest in live cells using structurally modulated fluorescent protein chromophores. Combining photophysical analysis, X-ray crystallography, and theoretical calculation, we show that fluorescence is triggered by inhibition of twisted-intramolecular charge transfer of these fluorophores in the rigid microenvironment of viscous solvent or protein aggregates. Bioorthogonal conjugation of the fluorophore to Halo-tag fused protein-of-interests allows for fluorogenic detection of both misfolded and aggregated species in live cells. Unlike other methods, our method is capable of detecting previously invisible misfolded soluble proteins. This work provides the first application of fluorescent protein chromophores to detect protein conformational collapse in live cells.

Entities: CellLine Chemical Disease Gene Mutation

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Year: 2018 PMID： 29883112 PMCID： PMC6258209 DOI： 10.1021/jacs.8b02176

Source DB: PubMed Journal: J Am Chem Soc ISSN： 0002-7863 Impact factor: 15.419

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