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FLEX: genetically encodable enzymatic fluorescence signal amplification using engineered peroxidase

Authors
Sharma, NirmaliJung, MinkyoMishra, Pratyush KumarMun, Ji YoungRhee, Hyun-Woo
Issue Date
Mar-2024
Publisher
Cell Press
Citation
Cell Chemical Biology, v.31, no.3, pp 502 - 513.e6
Journal Title
Cell Chemical Biology
Volume
31
Number
3
Start Page
502
End Page
513.e6
URI
http://scholarworks.bwise.kr/kbri/handle/2023.sw.kbri/1163
DOI
10.1016/j.chembiol.2024.02.007
ISSN
2451-9448
2451-9456
Abstract
Fluorescent tagging of biomolecules enables their sensitive detection during separation and determining their subcellular location. In this context, peroxidase-based reactions are actively utilized for signal amplification. To harness this potential, we developed a genetically encodable enzymatic fluorescence signal amplification method using APEX (FLEX). We synthesized a fluorescent probe, Jenfluor triazole (JFT1), which effectively amplifies and restricts fluorescence signals under fixed conditions, enabling fluorescence-based detection of subcellularly localized electron-rich metabolites. Moreover, JFT1 exhibited stable fluorescence signals even under osmium-treated and polymer-embedded conditions, which supported findings from correlative light and electron microscopy (CLEM) using APEX. Using various APEX-conjugated proteins of interest (POIs) targeted to different organelles, we successfully visualized their localization through FLEX imaging while effectively preserving organelle ultrastructures. FLEX provides insights into dynamic lysosome-mitochondria interactions upon exposure to chemical stressors. Overall, FLEX holds significant promise as a sensitive and versatile system for fluorescently detecting APEX2-POIs in multiscale biological samples.
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