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Development of a Time-Resolved Fluorometric Method for Observing Hybridization in Living Cells Using Fluorescence Resonance Energy Transfer

费斯特共振能量转移 荧光 接受者 自体荧光 荧光显微镜 化学 激光诱导荧光 荧光寿命成像显微镜 生物物理学 共振感应耦合 能量转移 细胞质 荧光光谱法 荧光互相关光谱 荧光团 共振荧光 激发 荧光计 分析化学(期刊) 材料科学 绿色荧光蛋白 化学物理 生物 生物化学 光学 色谱法 物理 凝聚态物理
作者
Akihiko Tsuji,Yoshihiro Sato,Masahiko Hirano,Takayuki Suga,Hiroyuki Koshimoto,Takeshi Taguchi,Shinji Ohsuka
出处
期刊:Biophysical Journal [Elsevier]
卷期号:81 (1): 501-515 被引量:55
标识
DOI:10.1016/s0006-3495(01)75717-7
摘要

We previously showed that a specific kind of mRNA (c-fos) was detected in a living cell under a microscope by introducing two fluorescently labeled oligodeoxynucleotides, each labeled with donor or acceptor, into the cytoplasm, making them hybridize to adjacent locations on c-fos mRNA, and taking images of fluorescence resonance energy transfer (FRET) (A. Tsuji, H. Koshimoto, Y. Sato, M. Hirano. Y. Sei-Iida, S. Kondo, and K. Ishibashi, 2000, Biophys. J. 78:3260–3274). On the formed hybrid, the distance between donor and acceptor becomes close and FRET occurs. To observe small numbers of mRNA in living cells using this method, it is required that FRET fluorescence of hybrid must be distinguished from fluorescence of excess amounts of non-hybridizing probes and from cell autofluorescence. To meet these requirements, we developed a time-resolved method using acceptor fluorescence decays. When a combination of a donor having longer fluorescence lifetime and an acceptor having shorter lifetime is used, the measured fluorescence decays of acceptors under FRET becomes slower than the acceptor fluorescence decay with direct excitation. A combination of Bodipy493/503 and Cy5 was selected as donor and acceptor. When the formed hybrid had a configuration where the target RNA has no single-strand part between the two fluorophores, the acceptor fluorescence of hybrid had a sufficiently longer delay to detect fluorescence of hybrid in the presence of excess amounts of non-hybridizing probes. Spatial separation of 10–12 bases between two fluorophores on the hybrid is also required. The decay is also much slower than cell autofluorescence, and smaller numbers of hybrid were detected with less interference of cell autofluorescence in the cytoplasm of living cells under a time-resolved fluorescence microscope with a time-gated function equipped camera. The present method will be useful when observing induced expressions of mRNA in living cells.

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