A fluorescent variant of a protein from the stony coral Montipora facilitates dual-color single-laser fluorescence cross-correlation spectroscopy

被引:0
|
作者
Takako Kogure
Satoshi Karasawa
Toshio Araki
Kenta Saito
Masataka Kinjo
Atsushi Miyawaki
机构
[1] Laboratory for Cell Function and Dynamics,
[2] Advanced Technology Development Group,undefined
[3] Brain Science Institute,undefined
[4] RIKEN,undefined
[5] 2-1 Hirosawa,undefined
[6] Wako-city,undefined
[7] Amalgaam Co.,undefined
[8] Ltd. 2-9-3 Itabashi,undefined
[9] Itabashi-ku,undefined
[10] Medical & Biological Laboratories Co.,undefined
[11] Ltd.,undefined
[12] 3-5-10 Marunouchi,undefined
[13] Naka-ku,undefined
[14] Research Institute for Electronic Science,undefined
[15] Hokkaido University,undefined
来源
Nature Biotechnology | 2006年 / 24卷
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摘要
Dual-color fluorescence cross-correlation spectroscopy (FCCS) is a promising technique for quantifying protein-protein interactions1,2,3,4,5. In this technique, two different fluorescent labels are excited and detected simultaneously within a common measurement volume. Difficulties in aligning two laser lines and emission crossover between the two fluorophores, however, make this technique complex. To overcome these limitations, we developed a fluorescent protein with a large Stokes shift. This protein, named Keima, absorbs and emits light maximally at 440 nm and 620 nm, respectively. Combining a monomeric version of Keima with cyan fluorescent protein allowed dual-color FCCS with a single 458-nm laser line and complete separation of the fluorescent protein emissions. This FCCS approach enabled sensitive detection of proteolysis by caspase-3 and the association of calmodulin with calmodulin-dependent enzymes. In addition, Keima and a spectral variant that emits maximally at 570 nm might facilitate simultaneous multicolor imaging with single-wavelength excitation.
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页码:577 / 581
页数:4
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