Literature DB >> 21886099

Investigating protein-protein interactions in living cells using fluorescence lifetime imaging microscopy.

Yuansheng Sun1, Richard N Day, Ammasi Periasamy.   

Abstract

Fluorescence lifetime imaging microscopy (FLIM) is now routinely used for dynamic measurements of signaling events inside living cells, including detection of protein-protein interactions. An understanding of the basic physics of fluorescence lifetime measurements is required to use this technique. In this protocol, we describe both the time-correlated single photon counting and the frequency-domain methods for FLIM data acquisition and analysis. We describe calibration of both FLIM systems, and demonstrate how they are used to measure the quenched donor fluorescence lifetime that results from Förster resonance energy transfer (FRET). We then show how the FLIM-FRET methods are used to detect the dimerization of the transcription factor CCAAT/enhancer binding protein-α in live mouse pituitary cell nuclei. Notably, the factors required for accurate determination and reproducibility of lifetime measurements are described. With either method, the entire protocol including specimen preparation, imaging and data analysis takes ∼2 d.

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Year:  2011        PMID: 21886099      PMCID: PMC3169422          DOI: 10.1038/nprot.2011.364

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  61 in total

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5.  Characterization of spectral FRET imaging microscopy for monitoring nuclear protein interactions.

Authors:  Ye Chen; Joshua P Mauldin; Richard N Day; Ammasi Periasamy
Journal:  J Microsc       Date:  2007-11       Impact factor: 1.758

6.  Characterization of an orange acceptor fluorescent protein for sensitized spectral fluorescence resonance energy transfer microscopy using a white-light laser.

Authors:  Yuansheng Sun; Cynthia F Booker; Sangeeta Kumari; Richard N Day; Mike Davidson; Ammasi Periasamy
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Review 7.  Fluorescence resonance energy transfer microscopy of localized protein interactions in the living cell nucleus.

Authors:  R N Day; A Periasamy; F Schaufele
Journal:  Methods       Date:  2001-09       Impact factor: 3.608

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Journal:  J Cell Biol       Date:  2003-03-03       Impact factor: 10.539

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  70 in total

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3.  Pulse-shaping based two-photon FRET stoichiometry.

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Review 4.  FRET-FLIM applications in plant systems.

Authors:  Christoph A Bücherl; Arjen Bader; Adrie H Westphal; Sergey P Laptenok; Jan Willem Borst
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5.  Thin-film tunable filters for hyperspectral fluorescence microscopy.

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6.  Multiphoton fluorescence lifetime imaging of chemotherapy distribution in solid tumors.

Authors:  Marjorie Carlson; Adrienne L Watson; Leah Anderson; David A Largaespada; Paolo P Provenzano
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7.  Video-rate two-photon excited fluorescence lifetime imaging system with interleaved digitization.

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8.  Direct interaction of CaVβ with actin up-regulates L-type calcium currents in HL-1 cardiomyocytes.

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9.  Evaluating the performance of time-gated live-cell microscopy with lanthanide probes.

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Review 10.  Recent trends in two-photon auto-fluorescence lifetime imaging (2P-FLIM) and its biomedical applications.

Authors:  Harsh Ranawat; Sagnik Pal; Nirmal Mazumder
Journal:  Biomed Eng Lett       Date:  2019-07-01
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