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Optical Lock-In Detection of FRET Using Synthetic and Genetically Encoded Optical Switches

机译:使用合成和遗传编码的光开关对FRET进行光学锁定检测

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摘要

The Förster resonance energy transfer (FRET) technique is widely used for studying protein interactions within live cells. The effectiveness and sensitivity of determining FRET, however, can be reduced by photobleaching, cross talk, autofluorescence, and unlabeled, endogenous proteins. We present a FRET imaging method using an optical switch probe, Nitrobenzospiropyran (NitroBIPS), which substantially improves the sensitivity of detection to <1% FRET efficiency. Through orthogonal optical control of the colorful merocyanine and colorless spiro states of the NitroBIPS acceptor, donor fluorescence can be measured both in the absence and presence of FRET in the same FRET pair in the same cell. A SNAP-tag approach is used to generate a green fluorescent protein-alkylguaninetransferase fusion protein (GFP-AGT) that is labeled with benzylguanine-NitroBIPS. In vivo imaging studies on this green fluorescent protein-alkylguaninetransferase (GFP-AGT) (NitroBIPS) complex, employing optical lock-in detection of FRET, allow unambiguous resolution of FRET efficiencies below 1%, equivalent to a few percent of donor-tagged proteins in complexes with acceptor-tagged proteins.
机译:Förster共振能量转移(FRET)技术被广泛用于研究活细胞内的蛋白质相互作用。但是,可通过光漂白,串扰,自发荧光和未标记的内源蛋白质降低测定FRET的有效性和敏感性。我们提出了使用光开关探针NitroBIPS(NitroBIPS)进行FRET成像的方法,该方法大大提高了检测灵敏度,使FRET效率小于1%。通过正交光学控制NitroBIPS受体的彩色花菁和无色螺环状态,可以在同一单元格中的同一FRET对中不存在FRET和存在FRET的情况下测量供体荧光。 SNAP标签方法用于生成绿色荧光蛋白-烷基鸟嘌呤转移酶融合蛋白(GFP-AGT),该蛋白被苄基鸟嘌呤-NitroBIPS标记。对这种绿色荧光蛋白-烷基鸟嘌呤转移酶(GFP-AGT)(NitroBIPS)复合物的体内成像研究,采用FRET的光学锁定检测,可以将FRET效率明确地分辨为低于1%,相当于供体标签蛋白的百分之几与受体标记的蛋白复合。

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