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Direct Quantification of Fusion Rate Reveals a Distal Role for AS160 in Insulin-stimulated Fusion of GLUT4 Storage Vesicles

机译:直接量化融合率揭示了AS160在治疗中的重要作用 胰岛素刺激的GLUT4存储融合 囊泡

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摘要

Insulin-stimulated GLUT4 translocation to the plasma membrane constitutes a key process for blood glucose control. However, convenient and robust assays to monitor this dynamic process in real time are lacking, which hinders current progress toward elucidation of the underlying molecular events as well as screens for drugs targeting this particular pathway. Here, we have developed a novel dual colored probe to monitor the translocation process of GLUT4 based on dual color fluorescence measurement. We demonstrate that this probe is more than an order of magnitude more sensitive than the current technology for detecting fusion events from single GLUT4 storage vesicles (GSVs). A small fraction of fusion events were found to be of the “kiss-and-run” type. For the first time, we show that insulin stimulation evokes a ∼40-fold increase in the fusion of GSVs in 3T3-L1 adipocytes, compared with basal conditions. The probe can also be used to monitor the prefusion behavior of GSVs. By quantifying both the docking and fusion rates simultaneously, we demonstrate a proportional inhibition in both docking and fusion of GSVs by a dominant negative mutant of AS160, indicating a role for AS160 in the docking of GSVs but not in the regulation of GSV fusion after docking.
机译:胰岛素刺激的GLUT4易位至质膜是控制血糖的关键过程。然而,缺乏实时监测该动态过程的方便和鲁棒的测定法,这阻碍了目前向阐明潜在分子事件以及筛选针对该特定途径的药物的进展。在这里,我们开发了一种新型的双色探针,可基于双色荧光测量来监测GLUT4的转运过程。我们证明,该探针比目前用于检测单个GLUT4储存囊泡(GSV)融合事件的技术的灵敏度高出一个数量级。发现一小部分融合事件属于“接吻运行”类型。我们首次显示,与基础条件相比,胰岛素刺激引起3T3-L1脂肪细胞中GSV融合的增加约40倍。该探针还可用于监测GSV的预融合行为。通过同时量化对接和融合率,我们证明了AS160的显性负突变体对GSV的对接和融合均具有成比例的抑制作用,表明AS160在GSV的对接中而不是在对GSV的调节中起作用 对接后融合。

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