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Spatial proteomic and phospho-proteomic organization in three prototypical cell migration modes

机译:三种典型细胞迁移模式下的空间蛋白质组学和磷酸化蛋白质组学

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Background Tight spatio-temporal signaling of cytoskeletal and adhesion dynamics is required for localized membrane protrusion that drives directed cell migration. Different ensembles of proteins are therefore likely to get recruited and phosphorylated in membrane protrusions in response to specific cues. Results Here, we use an assay that allows to biochemically purify extending protrusions of cells migrating in response to three prototypical receptors: integrins, recepor tyrosine kinases and G-coupled protein receptors. Using quantitative proteomics and phospho-proteomics approaches, we provide evidence for the existence of cue-specific, spatially distinct protein networks in the different cell migration modes. Conclusions The integrated analysis of the large-scale experimental data with protein information from databases allows us to understand some emergent properties of spatial regulation of signaling during cell migration. This provides the cell migration community with a large-scale view of the distribution of proteins and phospho-proteins regulating directed cell migration.
机译:背景技术对于驱动定向细胞迁移的局部膜突出,需要细胞骨架和粘附动力学的紧密时空信号传递。因此,响应特定的信号,可能会在膜突出物中募集不同的蛋白质整体并将其磷酸化。结果在这里,我们使用一种检测方法,该方法可以生化纯化迁移的细胞延伸突起,以响应三种原型受体:整联蛋白,recepor酪氨酸激酶和G偶联蛋白受体。使用定量蛋白质组学和磷酸化蛋白质组学方法,我们提供了在不同细胞迁移模式下存在提示特异性,空间上不同的蛋白质网络的证据。结论对大规模实验数据与数据库蛋白质信息的综合分析使我们能够了解细胞迁移过程中信号空间调节的一些新兴特性。这为细胞迁移群落提供了调节定向细胞迁移的蛋白质和磷酸蛋白分布的大规模视图。

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