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A Highlights from MBoC Selection: Live-cell multiphoton fluorescence correlation spectroscopy with an improved large Stokes shift fluorescent protein

机译:MBoC选择的亮点:具有改进的大型Stokes位移荧光蛋白的活细胞多光子荧光相关光谱

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We report an improved variant of mKeima, a monomeric long Stokes shift red fluorescent protein, hmKeima8.5. The increased intracellular brightness and large Stokes shift (~180 nm) make it an excellent partner with teal fluorescent protein (mTFP1) for multiphoton, multicolor applications. Excitation of this pair by a single multiphoton excitation wavelength (MPE, 850 nm) yields well-separable emission peaks (~120-nm separation). Using this pair, we measure homo- and hetero-oligomerization interactions in living cells via multiphoton excitation fluorescence correlation spectroscopy (MPE-FCS). Using tandem dimer proteins and small-molecule inducible dimerization domains, we demonstrate robust and quantitative detection of intracellular protein–protein interactions. We also use MPE-FCCS to detect drug–protein interactions in the intracellular environment using a Coumarin 343 (C343)-conjugated drug and hmKeima8.5 as a fluorescence pair. The mTFP1/hmKeima8.5 and C343/hmKeima8.5 combinations, together with our calibration constructs, provide a practical and broadly applicable toolbox for the investigation of molecular interactions in the cytoplasm of living cells.
机译:我们报告mKeima,单体长斯托克斯移红色荧光蛋白hmKeima8.5的改进的变体。增加的细胞内亮度和大的斯托克斯位移(〜180 nm)使它成为蓝绿色荧光蛋白(mTFP1)的出色搭档,适用于多光子,多色应用。用单个多光子激发波长(MPE,850 nm)激发该对离子,可产生可分离的发射峰(间隔约120 nm)。使用这一对,我们通过多光子激发荧光相关光谱法(MPE-FCS)测量活细胞中的均聚和异聚反应。使用串联二聚体蛋白和小分子可诱导的二聚化结构域,我们证明了对细胞内蛋白-蛋白相互作用的可靠和定量检测。我们还使用MPE-FCCS使用结合了香豆素343(C343)的药物和hmKeima8.5作为荧光对来检测细胞内环境中的药物-蛋白质相互作用。 mTFP1 / hmKeima8.5和C343 / hmKeima8.5的组合,以及我们的校准构建物,为研究活细胞细胞质中的分子相互作用提供了一种实用且广泛适用的工具箱。

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