Spectrally and spatially resolved fluorescence lifetime imaging in living cells: TRPV4-microfilament interactions |
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| Authors: | Ramadass Radhan Becker Daniel Jendrach Marina Bereiter-Hahn Jürgen |
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| Affiliation: | Kinematic Cell Research Group, Institute for Cell Biology and Neuroscience, JW Goethe University, Max-von-Laue-Strasse 9, D-60438 Frankfurt/Main, Germany. ramadass@bio.uni-frankfurt.de |
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| Abstract: | Time- and space-correlated single photon counting method has been used to demonstrate the interactions of cation channel "transient receptor potential vanilloid 4" (TRPV4) and microfilaments. Living cells co-expressing TRPV4-CFP and actin-YFP, when excited for the donor molecules (CFP) exhibited an emission peak at 527 nm and decrease of the lifetime in the wavelength band 460-490 nm; corresponding to resonance energy transfer to YFP. CFP fluorescence decay was fitted best by a dual mode decay model. Considering the average lifetime of the donor, both in the presence and absence of acceptor yielded an apparent FRET efficiency of approximately 20%. This is rather high placing the minimum distance of chromophores in the two fluorescent proteins in the range of 4 nm. Thus, this study shows for the first time that TRPV4 and actin intimately associate within living cells. The significance of this finding for cell volume regulation is highlighted. |
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| Keywords: | TRPV4 Actin Regulatory volume decrease Osmoregulation FLIM Time-resolved FRET Single photon counting CHO cells CFP YFP Fluorescent proteins Decay associated spectra Spectrally resolved fluorescence decays |
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