Tetrazine‐Isonitrile Bioorthogonal Fluorogenic Reactions Enable Multiplex Labeling and Wash‐Free Bioimaging of Live Cells

Author:

Deng Yingqiao1,Shen Tianruo2ORCID,Yu Xinyu1,Li Jie1,Zou Peixuan34,Gong Qiyong1,Zheng Yongxiang34,Sun Hongbao1ORCID,Liu Xiaogang2ORCID,Wu Haoxing14ORCID

Affiliation:

1. Department of Radiology and Huaxi MR Research Center (HMRRC) Functional and Molecular Imaging Key Laboratory of Sichuan Province and Frontiers Science Center for Disease Related Molecular Network West China Hospital Sichuan University Huaxi Research Building, 001 4th Keyuan Road 610041 Chengdu China

2. Science, Mathematics and Technology Cluster Singapore University of Technology and Design 8 Somapah Road 487372 Singapore Singapore

3. Department of Biopharmaceutics West China School of Pharmacy Sichuan University No.17 People's South Road 610041 Chengdu China

4. Key Laboratory of Drug-Targeting and Drug Delivery System of the Education Ministry Sichuan Engineering Laboratory for Plant-Sourced Drug and Sichuan Research Center for Drug Precision Industrial Technology West China School of Pharmacy Sichuan University No.17 People's South Road 610041 Chengdu China

Abstract

AbstractDeveloping fluorogenic probes for simultaneous live cell labeling of multiple targets is crucial for understanding complex cellular events. The emerging [4+1] cycloaddition between tetrazine and isonitriles holds promise as a bioorthogonal tool, yet existing tetrazine probes lack reactivity and fluorogenicity. Here, we present the development of a series of tetrazine‐functionalized bioorthogonal probes. By incorporating pyrazole adducts into the fluorophore scaffolds, the post‐reacted probes displayed remarkable fluorescence turn‐on ratios, up to 3184‐fold. Moreover, these modifications are generalizable to various fluorophores, enabling a broad emission range from 473 to 659 nm. Quantum chemical calculations further elucidate the turn‐on mechanisms. These probes enable the simultaneous labeling of multiple targets in live cells, without the need for a washing step. Consequently, our findings pave the way for advanced multiplex imaging and detection techniques for cellular studies.

Funder

National Key Research and Development Program of China

National Natural Science Foundation of China

Publisher

Wiley

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