Flaring Inflammation and ER Stress by an Organelle‐Specific Fluorescent Cage

Author:

Fakim Aliyah1,Maatouk Batoul I.1,Maiti Bappa1,Dey Avishek1,Alotaiby Shahad H.1,Moosa Basem A.1,Lin Weibin1,Khashab Niveen M.1ORCID

Affiliation:

1. Chemistry Program Physical Science and Engineering Division King Abdullah University of Science and Technology (KAUST) Thuwal 23955–6900 Saudi Arabia

Abstract

AbstractThe endoplasmic reticulum (ER) plays an important role in protein synthesis and its disruption can cause protein unfolding and misfolding. Accumulation of such proteins leads to ER stress, which ultimately promotes many diseases. Routine screening of ER activity in immune cells can flag serious conditions at early stages, but the current clinically used bio‐probes have limitations. Herein, an ER‐specific fluorophore based on a biocompatible benzothiadiazole‐imine cage (BTD‐cage) with excellent photophysical properties is developed. The cage outperforms commercially available ER stains in long‐term live cell imaging with no fading or photobleaching over time. The cage is responsive to different levels of ER stress where its fluorescence increases accordingly. Incorporating the bio‐probe into an immune disorder model, a 6‐, 21‐, and 48‐fold increase in intensity is shown in THP‐1, Raw 246.7, and Jurkat cells, respectively (within 15 min). These results strongly support that this system can be used for rapid visual and selective detection of ER stress. It is envisaged that tailoring molecular interactions and molecular recognition using supramolecular improved fluorophores can expand the library of biological probes for enhanced selectivity and targetability toward cellular organelles.

Publisher

Wiley

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