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High throughput FRET analysis of protein–protein interactions by slide‐based imaging laser scanning cytometry
Author(s) -
Szalóki Nikoletta,
DoanXuan Quang Minh,
Szöllősi János,
Tóth Katalin,
Vámosi György,
Bacsó Zsolt
Publication year - 2013
Publication title -
cytometry part a
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.316
H-Index - 90
eISSN - 1552-4930
pISSN - 1552-4922
DOI - 10.1002/cyto.a.22315
Subject(s) - cytometry , förster resonance energy transfer , throughput , laser scanning , flow cytometry , laser , biophysics , computational biology , nanotechnology , computer science , fluorescence , biology , materials science , microbiology and biotechnology , optics , physics , telecommunications , wireless
Laser scanning cytometry (LSC) is a slide‐based technique combining advantages of flow and image cytometry: automated, high‐throughput detection of optical signals with subcellular resolution. Fluorescence resonance energy transfer (FRET) is a spectroscopic method often used for studying molecular interactions and molecular distances. FRET has been measured by various microscopic and flow cytometric techniques. We have developed a protocol for a commercial LSC instrument to measure FRET on a cell‐by‐cell or pixel‐by‐pixel basis on large cell populations, which adds a new modality to the use of LSC. As a reference sample for FRET, we used a fusion protein of a single donor and acceptor (ECFP‐EYFP connected by a seven‐amino acid linker) expressed in HeLa cells. The FRET efficiency of this sample was determined via acceptor photobleaching and used as a reference value for ratiometric FRET measurements. Using this standard allowed the precise determination of an important parameter (the alpha factor, characterizing the relative signal strengths from a single donor and acceptor molecule), which is indispensable for quantitative FRET calculations in real samples expressing donor and acceptor molecules at variable ratios. We worked out a protocol for the identification of adherent, healthy, double‐positive cells based on light‐loss and fluorescence parameters, and applied ratiometric FRET equations to calculate FRET efficiencies in a semi‐automated fashion. To test our protocol, we measured the FRET efficiency between Fos‐ECFP and Jun‐EYFP transcription factors by LSC, as well as by confocal microscopy and flow cytometry, all yielding nearly identical results. Our procedure allows for accurate FRET measurements and can be applied to the fast screening of protein interactions. A pipeline exemplifying the gating and FRET analysis procedure using the CellProfiler software has been made accessible at our web site. © 2013 International Society for Advancement of Cytometry