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Single-cell FRET imaging of transferrin receptor trafficking dynamics by Sfp-catalyzed, site-specific protein labeling

机译:Sfp催化的位点特异性蛋白标记对转铁蛋白受体运输动力学的单细胞FRET成像

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摘要

Fluorescence imaging of living cells depends on an efficient and specific method for labeling the target cellular protein with fluorophores. Here we show that Sfp phosphopantetheinyl transferase-catalyzed protein labeling is suitable for fluorescence imaging of membrane proteins that spend at least part of their membrane trafficking cycle at the cell surface. In this study, transferrin receptor 1 (TfR1) was fused to peptide carrier protein (PCP), and the TfR1-PCP fusion protein was specifically labeled with fluorophore Alexa 488 by Sfp. The trafficking of transferrin-TfR1-PCP complex during the process of transferrin-mediated iron uptake was imaged by fluorescence resonance energy transfer between the fluorescently labeled transferrin ligand and TfR1 receptor. We thus demonstrated that Sfp-catalyzed small molecule labeling of the PCP tag represents a practical and efficient tool for molecular imaging studies in living cells.
机译:活细胞的荧光成像取决于用荧光团标记靶细胞蛋白的有效且特定的方法。在这里,我们显示Sfp磷酸泛肽基转移酶催化的蛋白质标记适用于膜蛋白的荧光成像,该膜蛋白至少将其膜运输周期的一部分花费在细胞表面。在这项研究中,转铁蛋白受体1(TfR1)与肽载体蛋白(PCP)融合,并且TfR1-PCP融合蛋白被Sfp标记为荧光团Alexa 488。通过荧光标记的转铁蛋白配体和TfR1受体之间的荧光共振能量转移,对转铁蛋白-TfR1-PCP复合物在运铁蛋白介导的铁摄取过程中的运输进行了成像。因此,我们证明了PCP标签的Sfp催化小分子标记代表了活细胞分子成像研究的实用和有效工具。

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