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Breaking the color barrier - a multi-selective antibody reporter offers innovative strategies of fluorescence detection

机译:打破颜色屏障 - 一种多选择性抗体记者提供荧光检测的创新策略

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A novel bi-partite fluorescence platform exploits the high affinity and selectivity of antibody scaffolds to capture and activate small-molecule fluorogens. In this report, we investigated the property of multiselectivity activation by a single antibody against diverse cyanine family fluorogens. Our fluorescence screen identified three cellimpermeant fluorogens, each with unique emission spectra (blue, green and red) and nanomolar affinities. Most importantly, as a protein fusion tag to G-protein-coupled receptors, the antibody biosensor retained full activity-displaying bright fluorogen signals with minimal background on live cells. Because fluorogen-activating antibodies interact with their target ligands via non-covalent interactions, we were able to perform advanced multi-color detection strategies on live cells, previously difficult or impossible with conventional reporters. We found that by fine-tuning the concentrations of the different color fluorogen molecules in solution, a user may interchange the fluorescence signal (onset versus offset), execute real-time signal exchange via fluorogen competition, measure multi-channel fluorescence via colabeling, and assess real-time cell surface receptor traffic via pulsechase experiments. Thus, here we inform of an innovative reporter technology based on tri-color signal that allows user-defined fluorescence tuning in live-cell applications.
机译:一种新型双墩荧光平台利用抗体支架的高亲和力和选择性,以捕获和激活小分子氟乙烯。在本报告中,我们调查了单抗体对不同型青霉素家族氟苯的多元化活化的性质。我们的荧光筛网鉴定了三种细胞哌米,每种荧光剂,每种氟化物均具有独特的发射光谱(蓝色,绿色和红色)和纳摩尔亲态。最重要的是,作为G蛋白偶联受体的蛋白质融合标签,抗体生物传感器保留了具有在活细胞上具有最小背景的明亮荧光信号。因为荧光激活抗体通过非共价相互作用与其靶配体相互作用,所以我们能够对活细胞进行先进的多色检测策略,以前与传统记者难以或不可能。我们发现,通过微调溶液中不同颜色荧光分子的浓度,使用者可以通过荧光竞争来交换荧光信号(起始与偏移),通过荧光竞争来执行实时信号交换,通过COLABELING测量多通道荧光,和通过脉冲酶实验评估实时细胞表面受体交通。因此,在这里,我们基于三色信号通知创新的报告技术,允许在实时电池应用中使用用户定义的荧光调整。

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