4.6 Article

Fluorogenic affinity label for the facile, rapid imaging of proteins in live cells

Journal

ORGANIC & BIOMOLECULAR CHEMISTRY
Volume 7, Issue 19, Pages 3969-3975

Publisher

ROYAL SOC CHEMISTRY
DOI: 10.1039/b907664f

Keywords

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Funding

  1. NIH [CA073808]
  2. NSF Graduate Research Fellowship
  3. Chemistry-Biology Interface Training [GM008505]
  4. ACS Division of Organic Chemistry Fellowship
  5. the Genentech Foundation
  6. Biotechnology Training [GM008349]
  7. Barry M. Goldwater Scholarship and a Hilldale Undergraduate/Faculty Research Fellowship
  8. NMRFAM [P41RR02301]
  9. NATIONAL CANCER INSTITUTE [R01CA073808] Funding Source: NIH RePORTER
  10. NATIONAL CENTER FOR RESEARCH RESOURCES [P41RR002301] Funding Source: NIH RePORTER
  11. NATIONAL INSTITUTE OF GENERAL MEDICAL SCIENCES [T32GM008349, T32GM008505] Funding Source: NIH RePORTER

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Haloalkane dehalogenase (HD) catalyzes the hydrolysis of haloalkanes via a covalent enzyme-substrate intermediate. Fusing a target protein to an HD variant that cannot hydrolyze the intermediate enables labeling of the target protein with a haloalkane in cellulo. The utility of extant probes is hampered, however, by background fluorescence as well as limited membrane permeability. Here, we report on the synthesis and use of a fluorogenic affinity label that, after unmasking by an intracellular esterase, labels an HD variant in cellulo. Labeling is rapid and specific, as expected from the reliance upon enzymic catalysts and the high membrane permeance of the probe both before and after unmasking. Most notably, even high concentrations of the fluorogenic affinity label cause minimal background fluorescence without a need to wash the cells. We envision that such fluorogenic affinity labels, which enlist catalysis by two cellular enzymes, will find utility in pulse-chase experiments, high-content screening, and numerous other protocols.

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