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Single-cell proteomic chip for profiling intracellular signaling pathways in single tumor cells

机译:单细胞蛋白质组学芯片用于分析单个肿瘤细胞中的细胞内信号通路

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摘要

We describe a microchip designed to quantify the levels of a dozen cytoplasmic and membrane proteins from single cells. We use the platform to assess protein–protein interactions associated with the EGF-receptor-mediated PI3K signaling pathway. Single-cell sensitivity is achieved by isolating a defined number of cells (n = 0–5) in 2 nL volume chambers, each of which is patterned with two copies of a miniature antibody array. The cells are lysed on-chip, and the levels of released proteins are assayed using the antibody arrays. We investigate three isogenic cell lines representing the cancer glioblastoma multiforme, at the basal level, under EGF stimulation, and under erlotinib inhibition plus EGF stimulation. The measured protein abundances are consistent with previous work, and single-cell analysis uniquely reveals single-cell heterogeneity, and different types and strengths of protein–protein interactions. This platform helps provide a comprehensive picture of altered signal transduction networks in tumor cells and provides insight into the effect of targeted therapies on protein signaling networks.
机译:我们描述了一种微芯片,旨在量化单个细胞中十几种细胞质和膜蛋白的水平。我们使用该平台评估与EGF受体介导的PI3K信号通路相关的蛋白质相互作用。通过在2个nL体积的腔室中隔离一定数量的细胞(n = 0-5),即可实现单细胞敏感性,每个腔室均以两个副本的微型抗体阵列进行图案化。将细胞裂解在芯片上,并使用抗体阵列测定释放蛋白的水平。我们在基础水平上,在EGF刺激下以及在厄洛替尼抑制加EGF刺激下研究了三种代表癌细胞恶性胶质母细胞瘤的同基因细胞系。测得的蛋白质丰度与以前的工作一致,并且单细胞分析独特地揭示了单细胞异质性以及蛋白质与蛋白质相互作用的不同类型和强度。该平台可帮助您全面了解肿瘤细胞中信号转导网络的变化,并深入了解靶向疗法对蛋白质信号网络的影响。

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