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NRhFluors: Quantitative Revealing the Interaction between Protein Homeostasis and Mitochondria Dysfunction via Fluorescence Lifetime Imaging. | LitMetric

NRhFluors: Quantitative Revealing the Interaction between Protein Homeostasis and Mitochondria Dysfunction via Fluorescence Lifetime Imaging.

ACS Cent Sci

Department of Chemistry and Research Center for Industries of the Future, Westlake University, 600 Dunyu Road, Hangzhou 310030, Zhejiang China.

Published: April 2024

AI Article Synopsis

  • Degenerative diseases are linked to protein conformation changes, making it essential to have tools for detecting these changes in cells.
  • A new near-infrared AIE probe based on rhodamine fluorophores has been developed, showing dual responses in fluorescence to local viscosity changes, and its activation is influenced by the viscosity environment.
  • This probe can be used with fluorescence lifetime imaging (FLIM) to monitor protein changes in cells, demonstrating effects like mitochondrial dysfunction and protein expression reduction, providing insights for understanding disease mechanisms and potential therapies.

Article Abstract

Degenerative diseases are closely related to the changes of protein conformation beyond the steady state. The development of feasible tools for quantitative detection of changes in the cellular environment is crucial for investigating the process of protein conformational variations. Here, we have developed a near-infrared AIE probe based on the rhodamine fluorophore, which exhibits dual responses of fluorescence intensity and lifetime to local viscosity changes. Notably, computational analysis reveals that NRhFluors fluorescence activation is due to inhibition of the RACI mechanism in viscous environment. In the chemical regulation of rhodamine fluorophores, we found that variations of electron density distribution can effectively regulate CI states and achieve fluorescence sensitivity of NRhFluors. In addition, combined with the AggTag method, the lifetime of probe A9-Halo exhibits a positive correlation with viscosity changes. This analytical capacity allows us to quantitatively monitor protein conformational changes using fluorescence lifetime imaging (FLIM) and demonstrate that mitochondrial dysfunction leads to reduced protein expression in HEK293 cells. In summary, this work developed a set of near-infrared AIE probes activated by the RACI mechanism, which can quantitatively detect cell viscosity and protein aggregation formation, providing a versatile tool for exploring disease-related biological processes and therapeutic approaches.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11046461PMC
http://dx.doi.org/10.1021/acscentsci.3c01532DOI Listing

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