Organelle membrane-specific chemical labeling and dynamic imaging in living cells

Lipids play crucial roles as structural elements, signaling molecules and material transporters in cells. However, the functions and dynamics of lipids within cells remain unclear because of a lack of methods to selectively label lipids in specific organelles and trace their movement by live-cell im...

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Veröffentlicht in:Nature chemical biology 2020-12, Vol.16 (12), p.1361-1367
Hauptverfasser: Tamura, Tomonori, Fujisawa, Alma, Tsuchiya, Masaki, Shen, Yuying, Nagao, Kohjiro, Kawano, Shin, Tamura, Yasushi, Endo, Toshiya, Umeda, Masato, Hamachi, Itaru
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Sprache:eng
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Zusammenfassung:Lipids play crucial roles as structural elements, signaling molecules and material transporters in cells. However, the functions and dynamics of lipids within cells remain unclear because of a lack of methods to selectively label lipids in specific organelles and trace their movement by live-cell imaging. We describe here a technology for the selective labeling and fluorescence imaging (microscopic or nanoscopic) of phosphatidylcholine in target organelles. This approach involves the metabolic incorporation of azido-choline, followed by a spatially limited bioorthogonal reaction that enables the visualization and quantitative analysis of interorganelle lipid transport in live cells. More importantly, with live-cell imaging, we obtained direct evidence that the autophagosomal membrane originates from the endoplasmic reticulum. This method is simple and robust and is thus powerful for real-time tracing of interorganelle lipid trafficking. Imaging of phosphatidylcholine, sphingomyelin and their interorganelle lipid transport in live cells, using azido-choline and a spatially limited bioorthogonal tag, suggests that autophagosomal membranes originate from the ER.
ISSN:1552-4450
1552-4469
DOI:10.1038/s41589-020-00651-z