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Real Time Fluorescence Imaging of Plcγ Translocation and Its Interaction with the Epidermal Growth Factor Receptor

机译:Plcγ转运的实时荧光成像及其与表皮生长因子受体的相互作用

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The translocation of fluorescently tagged PLCγ and requirements for this process in cells stimulated with EGF were analyzed using real time fluorescence microscopy applied for the first time to monitor growth factor receptor–effector interactions. The translocation of PLCγ to the plasma membrane required the functional Src homology 2 domains and was not affected by mutations in the pleckstrin homology domain or inhibition of phosphatidylinositol (PI) 3-kinase. An array of domains specific for PLCγ isoforms was sufficient for this translocation. The dynamics of translocation to the plasma membrane and redistribution of PLCγ, relative to localization of the EGF receptor and PI 4,5-biphosphate (PI 4,5-P2), were shown. Colocalization with the receptor was observed in the plasma membrane and in membrane ruffles where PI 4,5-P2 substrate could also be visualized. At later times, internalization of PLCγ, which could lead to separation from the substrate, was observed. The data support a direct binding of PLCγ to the receptor as the main site of the plasma membrane recruitment. The presence of PLCγ in membrane structures and its access to the substrate appear to be transient and are followed by a rapid incorporation into intracellular vesicles, leading to downregulation of the PLC activity.
机译:荧光标记的PLCγ的易位性和该过程在用EGF刺激的细胞中的要求已通过首次用于监测生长因子受体-效应子相互作用的实时荧光显微镜分析。 PLCγ向质膜的转运需要功能性Src同源性2域,不受pleckstrin同源性域突变或磷脂酰肌醇(PI)3-激酶抑制的影响。 PLCγ亚型特异的结构域阵列足以实现这种移位。显示了相对于EGF受体和PI 4,5-双磷酸酯(PI 4,5-P2)的定位,向质膜移位和PLCγ重新分布的动力学。在质膜和膜褶中观察到了与受体的共定位,其中PI 4,5-P2底物也可以被观察到。稍后,观察到PLCγ的内在化,这可能导致与底物的分离。数据支持PLCγ与受体直接结合,作为质膜募集的主要部位。膜结构中PLCγ的存在及其与基质的接触似乎是短暂的,随后迅速掺入细胞内囊泡,导致PLC活性下调。

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