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Evaluating Riboglow-FLIM probes for RNA sensing.
Sarfraz, Nadia; Shafik, Luke K; Stickelman, Zachary R; Shankar, Uma; Moscoso, Emilia; Braselmann, Esther.
Afiliación
  • Sarfraz N; Department of Chemistry, Georgetown University Washington District of Columbia USA esther.braselmann@georgetown.edu.
  • Shafik LK; Department of Chemistry, Georgetown University Washington District of Columbia USA esther.braselmann@georgetown.edu.
  • Stickelman ZR; Department of Chemistry, Georgetown University Washington District of Columbia USA esther.braselmann@georgetown.edu.
  • Shankar U; Department of Chemistry, Georgetown University Washington District of Columbia USA esther.braselmann@georgetown.edu.
  • Moscoso E; Department of Chemistry, Georgetown University Washington District of Columbia USA esther.braselmann@georgetown.edu.
  • Braselmann E; Department of Chemistry, Georgetown University Washington District of Columbia USA esther.braselmann@georgetown.edu.
RSC Chem Biol ; 5(2): 109-116, 2024 Feb 07.
Article en En | MEDLINE | ID: mdl-38333191
ABSTRACT
We recently developed Riboglow-FLIM, where we genetically tag and track RNA molecules in live cells through measuring the fluorescence lifetime of a small molecule probe that binds the RNA tag. Here, we systematically and quantitatively evaluated key elements of Riboglow-FLIM that may serve as the foundation for Riboglow-FLIM applications and further tool development efforts. Our investigation focused on measuring changes in fluorescence lifetime of representative Riboglow-FLIM probes with different linkers and fluorophores in different environments. In vitro measurements revealed distinct lifetime differences among the probe variants as a result of different linker designs and fluorophore selections. To expand on the platform's versatility, probes in a wide variety of mammalian cell types were examined using fluorescence lifetime imaging microscopy (FLIM), and possible effects on cell physiology were evaluated by metabolomics. The results demonstrated that variations in lifetime were dependent on both probe and cell type. Interestingly, distinct differences in lifetime values were observed between cell lines, while no overall change in cell health was measured. These findings underscore the importance of probe selection and cellular environment when employing Riboglow-FLIM for RNA detection, serving as a foundation for future tool development and applications across diverse fields and biological systems.

Texto completo: 1 Colección: 01-internacional Base de datos: MEDLINE Idioma: En Revista: RSC Chem Biol Año: 2024 Tipo del documento: Article

Texto completo: 1 Colección: 01-internacional Base de datos: MEDLINE Idioma: En Revista: RSC Chem Biol Año: 2024 Tipo del documento: Article
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