Fluorescence energy transfer measurements on cell surfaces: A critical comparison of steady‐state fluorimetric and flow cytometric methods

Abstract: The energy transfer efficiency E was measured between fluorescein-conjugated concanavalin A (Con A) and rhodamine-conjugated Con A bound to homogeneous tissue culture cells, the HK22 murine lymphoma cell line. Results from a flow cytometric energy transfer method (FCET) and two different steady-state fluorimeter methods were compared. The data were found to be in close agreement after careful correction of the steady-state fluorimetric measurements for contributions from dissociating ligand. The biological var… Show more

“…Donor and acceptor emissions were separated by a 525-nm dichroic mirror and were detected through 487/37-nm and 560/70-nm bandpass mirrors, respectively. Donor, acceptor, and FRET intensities were recorded as described previously (17,18). Briefly, two fluorescence intensities were detected for the donor excitation at 457 nm (donor channel I 1 , detection at 487 nm; acceptor channel I 2 , emission corresponding to the FRET channel at 560 nm), and one intensity was measured for the acceptor excitation at 514 nm (I 3 , acceptor emission at 560 nm).…”

“…Therefore, three independent measurements have to be taken that correspond to the donor (I 1 ), FRET (I 2 ), and acceptor (I 3 ) channels (17,18):…”

“…S 1 corrects for the overspill of donor fluorescence from I 1 to I 2 , S 3 for the overspill of donor fluorescence from I 1 to I 3 , and S 2 for the overspill of acceptor emission from I 3 to I 2 . The constants S 1 to S 3 are determined on single-labeled samples as described previously (17,18) and can be expressed by the following equations:…”

“…We previously reported one such method based on the combined detection of donor and acceptor fluorescence intensities in cells labeled with fluorescent ligands or antibodies using flow cytometry (17,18). Later, we established a similar method in fluorescence microscopy (19).…”

“…These methods require a factor, variably called a (17)(18)(19) or G (11,13), which relates the intensity lost on the donor side due to donor quenching to the enhanced emission of the acceptor due to sensitized emission. Methods for the determination of a have been reported for antibody-labeled cells in flow cytometry (17,18) and microscopy (19) and lately for VFP-expressing cells in microscopy (13). To the best of our knowledge, successful determination of a has not been reported for VFP-expressing cells using flow cytometry.…”

Novel calibration method for flow cytometric fluorescence resonance energy transfer measurements between visible fluorescent proteins

“…Donor and acceptor emissions were separated by a 525-nm dichroic mirror and were detected through 487/37-nm and 560/70-nm bandpass mirrors, respectively. Donor, acceptor, and FRET intensities were recorded as described previously (17,18). Briefly, two fluorescence intensities were detected for the donor excitation at 457 nm (donor channel I 1 , detection at 487 nm; acceptor channel I 2 , emission corresponding to the FRET channel at 560 nm), and one intensity was measured for the acceptor excitation at 514 nm (I 3 , acceptor emission at 560 nm).…”

“…Therefore, three independent measurements have to be taken that correspond to the donor (I 1 ), FRET (I 2 ), and acceptor (I 3 ) channels (17,18):…”

“…S 1 corrects for the overspill of donor fluorescence from I 1 to I 2 , S 3 for the overspill of donor fluorescence from I 1 to I 3 , and S 2 for the overspill of acceptor emission from I 3 to I 2 . The constants S 1 to S 3 are determined on single-labeled samples as described previously (17,18) and can be expressed by the following equations:…”

“…We previously reported one such method based on the combined detection of donor and acceptor fluorescence intensities in cells labeled with fluorescent ligands or antibodies using flow cytometry (17,18). Later, we established a similar method in fluorescence microscopy (19).…”

“…These methods require a factor, variably called a (17)(18)(19) or G (11,13), which relates the intensity lost on the donor side due to donor quenching to the enhanced emission of the acceptor due to sensitized emission. Methods for the determination of a have been reported for antibody-labeled cells in flow cytometry (17,18) and microscopy (19) and lately for VFP-expressing cells in microscopy (13). To the best of our knowledge, successful determination of a has not been reported for VFP-expressing cells using flow cytometry.…”

Novel calibration method for flow cytometric fluorescence resonance energy transfer measurements between visible fluorescent proteins

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