| Literature DB >> 33397937 |
Hongbao Fang1,2,3, Shanshan Geng1, Mingang Hao2, Qixin Chen2, Minglun Liu1, Chunyan Liu4, Zhiqi Tian2, Chengjun Wang5, Takanori Takebe4,6,7,8,9, Jun-Lin Guan2, Yuncong Chen10,11, Zijian Guo1,3, Weijiang He12,13, Jiajie Diao14.
Abstract
Zn2+ plays important roles in metabolism and signaling regulation. Subcellular Zn2+ compartmentalization is essential for organelle functions and cell biology, but there is currently no method to determine Zn2+ signaling relationships among more than two different organelles with one probe. Here, we report simultaneous Zn2+ tracking in multiple organelles (Zn-STIMO), a method that uses structured illumination microscopy (SIM) and a single Zn2+ fluorescent probe, allowing super-resolution morphology-correlated organelle identification in living cells. To guarantee SIM imaging quality for organelle identification, we develop a new turn-on Zn2+ fluorescent probe, NapBu-BPEA, by regulating the lipophilicity of naphthalimide-derived Zn2+ probes to make it accumulate in multiple organelles except the nucleus. Zn-STIMO with this probe shows that CCCP-induced mitophagy in HeLa cells is associated with labile Zn2+ enhancement. Therefore, direct organelle identification supported by SIM imaging makes Zn-STIMO a reliable method to determine labile Zn2+ dynamics in various organelles with one probe. Finally, SIM imaging of pluripotent stem cell-derived organoids with NapBu-BPEA demonstrates the potential of super-resolution morphology-correlated organelle identification to track biospecies and events in specific organelles within organoids.Entities:
Year: 2021 PMID: 33397937 DOI: 10.1038/s41467-020-20309-7
Source DB: PubMed Journal: Nat Commun ISSN: 2041-1723 Impact factor: 14.919