Picosecond-hetero-FRET microscopy to probe protein-protein interactions in live cells

被引:110
作者
Tramier, M
Gautier, I
Piolot, T
Ravalet, S
Kemnitz, K
Coppey, J
Durieux, C
Mignotte, V
Coppey-Moisan, M
机构
[1] Univ Paris 06, Inst Jacques Monod, UMR 7592 CNRS, F-75251 Paris 05, France
[2] Univ Paris 07, Inst Jacques Monod, UMR 7592 CNRS, F-75251 Paris 05, France
[3] EuroPhoton GMBH, D-12247 Berlin, Germany
[4] Maternite Port Royal, ICGM, Dept Hematol, F-75014 Paris, France
关键词
D O I
10.1016/S0006-3495(02)75357-5
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
By using a novel time- and space-correlated single-photon counting detector, we show that fluorescence resonance energy transfer (FRET) between cyan fluorescent protein (CFP) and yellow fluorescent protein (YFP) fused to herpes simplex virus thymidine kinase (TK) monomers can be used to reveal homodimerization of TK in the nucleus and cytoplasm of live cells. However, the quantification of energy transfer was limited by the intrinsic biexponential fluorescence decay of the donor CFP (lifetimes of 1.3 +/- 0.2 ns and 3.8 +/- 0.4 ns) and by the possibility of homodimer formation between two TK-CFP. In contrast, the heterodimerization of the transcriptional factor NF-E2 in the nucleus of live cells was quantified from the analysis of the fluorescence decays of GFP in terms of 1) FRET efficiency between GFP and DsRed chromophores fused to p45 and MafG, respectively, the two subunits of NF-E2 (which corresponds to an interchromophoric distance of 39 +/- 1 Angstrom); and 2) fractions of GFP-p45 bound to DsRed-MafG (constant in the nucleus, varying in the range of 20% to 70% from cell to cell). The picosecond resolution of the fluorescence kinetics allowed us to discriminate between very short lifetimes of immature green species of DsRed-MafG and that of GFP-p45 involved in FRET with DsRed-MafG.
引用
收藏
页码:3570 / 3577
页数:8
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