4.8 Article

Robust Packing of a Self-Assembling Iridium Complex via Endocytic Trafficking for Long-Term Lysosome Tracking

Journal

ANGEWANDTE CHEMIE-INTERNATIONAL EDITION
Volume 60, Issue 14, Pages 7597-7601

Publisher

WILEY-V C H VERLAG GMBH
DOI: 10.1002/anie.202015913

Keywords

bioinorganic chemistry; imaging agents; iridium; lysosome tracking; self-assembly-induced emission

Funding

  1. Proof-of-Concept program of OIST
  2. Takeda Science Foundation, Japan
  3. National Natural Science Foundation of China [21525105, 21701196]

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A novel lysosomal probe was designed and synthesized in this study, which self-assembles into stable network structures at extremely low concentrations, enabling long-term live cell imaging. This probe can efficiently label lysosomes in cells up to the 14th passage with minimal impact on luminescence intensity, and illuminated lysosomes are trackable using super-resolution imaging to study their response to cellular processes.
Live cell imaging of lysosome positioning and motility is critical to studying lysosome status and function for pharmacological interventions. To create a super stable lysosomal probe for long-term live cell imaging, we have designed and synthesized an aromatic-peptide-conjugated cyclometalated iridium(III) complex that emits light via pi-pi stacking oriented self-assembly in water at extremely low concentration. Through endocytic trafficking, self-assemblies are transformed from nanoparticles into sturdily packed networks that are stabilized in lysosomal acidic environment. Upon short time/low dose treatment of the iridium complex at passage 0, live cell lysosomal tracking is applicable beyond the 14th passage of cells with high labelling rate and a mild decline in luminescence intensity. The illuminated lysosomes are trackable using super-resolution imaging to study their response to cellular processes.

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