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Identification of new fluorescent protein fragments for bimolecular fluorescence complementation analysis under physiological conditions

机译:鉴定新的荧光蛋白片段,用于在生理条件下进行双分子荧光互补分析

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Protein-protein interactions play a pivotal role in coordinating many cellular processes. Determination of subcellular localization of interacting proteins and visualization of dynamic interactions in living cells are crucial to elucidate cellular functions of proteins. Using fluorescent proteins, we previously developed a bimolecular fluorescence complementation (BiFC) assay and a multicolor BiFC assay to visualize protein-protein interactions in living cells. However, the sensitivity of chromophore maturation of enhanced yellow fluorescent protein (YFP) to higher temperatures requires preincubation at lower temperatures prior to visualizing the BiFC signal. This could potentially limit their applications for the study of many signaling molecules. Here we report the identification of new fluorescent protein fragments derived from Venus and Cerulean for BiFC and multicolor BiFC assays under physiological culture conditions. More importantly, the newly identified combinations exhibit a 13-fold higher BiFC efficiency than originally identified fragments derived from YFP. Furthermore, the use of new combinations reduces the amount of plasmid required for transfection and shortens the incubation time, leading to a 2-fold increase in specific BiFC signals. These newly identified fluorescent protein fragments will facilitate the study of protein-protein interactions in living cells and whole animals under physiological conditions.
机译:蛋白质-蛋白质相互作用在协调许多细胞过程中起关键作用。相互作用蛋白亚细胞定位的确定和活细胞中动态相互作用的可视化对于阐明蛋白的细胞功能至关重要。使用荧光蛋白,我们先前开发了双分子荧光互补(BiFC)测定法和多色BiFC测定法以可视化活细胞中的蛋白质-蛋白质相互作用。但是,增强的黄色荧光蛋白(YFP)的发色团成熟度对较高温度的敏感性需要在可视化BiFC信号之前在较低温度下进行预培养。这可能会限制其在许多信号分子研究中的应用。在这里,我们报告了在生理培养条件下用于金银花和蓝宝石的新荧光蛋白片段的鉴定,用于BiFC和​​多色BiFC分析。更重要的是,新鉴定出的组合比原始鉴定出的源自YFP的片段展现出高13倍的BiFC效率。此外,使用新的组合可减少转染所需质粒的量并缩短孵育时间,从而导致特定BiFC信号增加2倍。这些新发现的荧光蛋白片段将有助于研究在生理条件下活细胞和整个动物体内的蛋白-蛋白相互作用。

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