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A Flow Cytometry-Based FRET Assay to Identify and Analyse Protein-Protein Interactions in Living Cells
Author(s) -
Carina Banning,
Jörg Votteler,
Dirk Hoffmann,
Herwig Koppensteiner,
Martin Warmer,
Rudolph Reimer,
Frank Kirchhoff,
Ulrich S. Schubert,
Joachim Hauber,
Michael Schindler
Publication year - 2010
Publication title -
plos one
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.99
H-Index - 332
ISSN - 1932-6203
DOI - 10.1371/journal.pone.0009344
Subject(s) - förster resonance energy transfer , flow cytometry , tetherin , protein–protein interaction , microbiology and biotechnology , biology , hek 293 cells , fluorescence microscope , plasma protein binding , human immunodeficiency virus (hiv) , computational biology , chemistry , virology , cell culture , viral envelope , fluorescence , genetics , physics , quantum mechanics
Background Försters resonance energy transfer (FRET) microscopy is widely used for the analysis of protein interactions in intact cells. However, FRET microscopy is technically challenging and does not allow assessing interactions in large cell numbers. To overcome these limitations we developed a flow cytometry-based FRET assay and analysed interactions of human and simian immunodeficiency virus (HIV and SIV) Nef and Vpu proteins with cellular factors, as well as HIV Rev multimer-formation. Results Amongst others, we characterize the interaction of Vpu with CD317 (also termed Bst-2 or tetherin), a host restriction factor that inhibits HIV release from infected cells and demonstrate that the direct binding of both is mediated by the Vpu membrane-spanning region. Furthermore, we adapted our assay to allow the identification of novel protein interaction partners in a high-throughput format. Conclusion The presented combination of FRET and FACS offers the precious possibility to discover and define protein interactions in living cells and is expected to contribute to the identification of novel therapeutic targets for treatment of human diseases.

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