Citation

  • Authors: Kaddoum, L., Magdeleine, E., Waldo, G. S., Joly, E., Cabantous, S.
  • Year: 2010
  • Journal: Biotechniques 49 727-8, 730, 732 passim
  • Applications: in vitro / DNA / jetPEI
  • Cell types:
    1. Name: HEK-293
      Description: Human embryonic kidney Fibroblast
      Known as: HEK293, 293
    2. Name: N2A
      Description: Murine neuroblastoma cells
      Known as: Neuro2A

Abstract

Although epitope tags are useful to detect intracellular proteins and follow their localization with antibodies, background and nonspecific staining often remain problematic. We describe a simple assay based on the split GFP complementation system. Proteins tagged with the 15-amino acid GFP 11 fragment are detected with a solution of the recombinant nonfluorescent complementary GFP 1-10 fragment to reconstitute a fluorescent GFP. In contrast to antibody-based staining methods, this one-step assay presents high specificity and very low background of fluorescence, thus conferring higher signal-to-noise ratios. We demonstrate that this new application of the split GFP tagging system facilitates detection of proteins displaying various subcellular localizations using flow cytometry and microscopy analysis.

Go to