4.6 Article

Deeper insight into protease-sensitive covalent-assembly fluorescent probes for practical biosensing applications

期刊

ORGANIC & BIOMOLECULAR CHEMISTRY
卷 17, 期 39, 页码 8918-8932

出版社

ROYAL SOC CHEMISTRY
DOI: 10.1039/c9ob01773a

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资金

  1. CNRS, Universite de Bourgogne
  2. Conseil Regional de Bourgogne through the Plan d'Actions Regional pour l'innovation (PARI) program
  3. Conseil Regional de Bourgogne through the Fonds Europeen de Developpement Regional (FEDER) program
  4. Burgundy region (FABER programme, PARI Action 6, SSTIC 6 Imagerie, instrumentation, chimie et applications biomedicales)
  5. Agence Nationale de la Recherche (ANR, AAPG 2018, PRCI LuminoManufacOligo) [ANR-18-CE07-0045-01]
  6. National Research Foundation Singapore (NRF, LuminoManufacOligo) [NRF2018-NRF-ANR035]
  7. GDR CNRS Agents d'Imagerie Moleculaire (AIM) 2037
  8. Agence Nationale de la Recherche (ANR) [ANR-18-CE07-0045] Funding Source: Agence Nationale de la Recherche (ANR)

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We report a rational and systematic study devoted to the structural optimisation of a novel class of protease-sensitive fluorescent probes that we recently reported (S. Debieu and A. Romieu, Org. Biomol. Chem., 2017, 15, 2575-2584), based on the covalent-assembly strategy and using the targeted enzyme penicillin G acylase as a model protease to build a fluorescent pyronin dye by triggering a biocompatible domino cyclisation-aromatisation reaction. The aim is to identify ad hoc probe candidate(s) that might combine fast/reliable fluorogenic turn-on response, full stability in complex biological media and ability to release a second molecule of interest (drug or second fluorescent reporter), for applications in disease diagnosis and therapy. We base our strategy on screening a set of active methylene compounds (C-nucleophiles) to convert the parent probe to various pyronin caged precursors bearing Michael acceptor moieties of differing reactivities. In vitro stability and fluorescent enzymatic assays combined with HPLC-fluorescence analyses provide data useful for defining the most appropriate structural features for these fluorogenic scaffolds depending on the specifications inherent to biological application (from biosensing to theranostics) for which they will be used.

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