4.6 Article

Fluorogenic label for biomolecular imaging

Journal

ACS CHEMICAL BIOLOGY
Volume 1, Issue 4, Pages 252-260

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/cb600132m

Keywords

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Funding

  1. NATIONAL CANCER INSTITUTE [R01CA073808] Funding Source: NIH RePORTER
  2. NATIONAL CENTER FOR RESEARCH RESOURCES [P41RR002301, S10RR013790] Funding Source: NIH RePORTER
  3. NCI NIH HHS [CA73808, R01 CA073808-08, R01 CA073808] Funding Source: Medline
  4. NCRR NIH HHS [S10 RR013790, RR13790, P41 RR002301, P41RR02301] Funding Source: Medline
  5. PHS HHS [08349] Funding Source: Medline

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Traditional small-molecule fluorophores are always fluorescent. This attribute can obscure valuable information in biological experiments. Here, we report on a versatile latent fluorophore that overcomes this limitation. At the core of the latent fluorophore is a derivative of rhodamine in which one nitrogen is modified as a urea. That modification enables rhodamine to retain half of its fluorescence while facilitating conjugation to a target molecule. The other nitrogen of rhodamine is modified with a trimethyl lock, which enables fluorescence to be unmasked fully by a single user-designated chemical reaction. An esterase-reactive latent fluorophore was synthesized in high yield and attached covalently to a cationic protein. The resulting conjugate was not fluorescent in the absence of esterases. The enzymatic activity of esterases in endocytic vesicles and the cytosol educed fluorescence, enabling the time-lapse imaging of endocytosis into live human cells and thus providing unprecedented spatiotemporal resolution of this process. The modular design of this fluorogenic label enables the facile synthesis of an ensemble of small-molecule probes for the illumination of numerous biochemical and cell biological processes.

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