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A NIR-Fluorochrome for Live Cell Dual Emission and Lifetime Tracking from the First Plasma Membrane Interaction to Subcellular and Extracellular Locales.
Booth, Eden; Garre, Massimiliano; Wu, Dan; Daly, Harrison C; O'Shea, Donal F.
Affiliation
  • Booth E; Department of Chemistry, Royal College of Surgeons in Ireland (RCSI), D02 PN40 Dublin, Ireland.
  • Garre M; Department of Chemistry, Royal College of Surgeons in Ireland (RCSI), D02 PN40 Dublin, Ireland.
  • Wu D; Department of Chemistry, Royal College of Surgeons in Ireland (RCSI), D02 PN40 Dublin, Ireland.
  • Daly HC; Department of Chemistry, Royal College of Surgeons in Ireland (RCSI), D02 PN40 Dublin, Ireland.
  • O'Shea DF; Department of Chemistry, Royal College of Surgeons in Ireland (RCSI), D02 PN40 Dublin, Ireland.
Molecules ; 29(11)2024 May 24.
Article de En | MEDLINE | ID: mdl-38893352
ABSTRACT
Molecular probes with the ability to differentiate between subcellular variations in acidity levels remain important for the investigation of dynamic cellular processes and functions. In this context, a series of cyclic peptide and PEG bio-conjugated dual near-infrared emissive BF2-azadipyrromethene fluorophores with maxima emissions at 720 nm (at pH > 6) and 790 nm (at pH < 5) have been developed and their aqueous solution photophysical properties determined. Their inter-converting emissions and fluorescence lifetime characteristics were exploited to track their spatial and temporal progression from first contact with the plasma membrane to subcellular locales to their release within extracellular vesicles. A pH-dependent reversible phenolate/phenol interconversion on the fluorophore controlled the dynamic changes in dual emission responses and corresponding lifetime changes. Live-cell confocal microscopy experiments in the metastatic breast cancer cell line MDA-MB-231 confirmed the usability of the dual emissive properties for imaging over prolonged periods. All three derivatives performed as probes capable of real-time continuous imaging of fundamental cellular processes such as plasma membrane interaction, tracking endocytosis, lysosomal/large acidic vesicle accumulation, and efflux within extracellular vesicles without perturbing cellular function. Furthermore, fluorescence lifetime imaging microscopy provided valuable insights regarding fluorophore progression through intracellular microenvironments over time. Overall, the unique photophysical properties of these fluorophores show excellent potential for their use as information-rich probes.
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Texte intégral: 1 Collection: 01-internacional Base de données: MEDLINE Sujet principal: Membrane cellulaire / Colorants fluorescents Limites: Humans Langue: En Journal: Molecules Sujet du journal: BIOLOGIA Année: 2024 Type de document: Article Pays d'affiliation: Irlande Pays de publication: Suisse

Texte intégral: 1 Collection: 01-internacional Base de données: MEDLINE Sujet principal: Membrane cellulaire / Colorants fluorescents Limites: Humans Langue: En Journal: Molecules Sujet du journal: BIOLOGIA Année: 2024 Type de document: Article Pays d'affiliation: Irlande Pays de publication: Suisse