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Mass Spectrometry-based Label-free Quantitative Proteomics To Study the Effect of 3PO Drug at Cellular Level

机译:基于质谱的无标记定量蛋白质组学,以研究3PO药物在细胞水平下的作用

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摘要

Human endothelial cells (ECs) have been employed to monitor the protein changes induced' by [3-(3-pyridiny1)-1-(4-pyridiny1)-2-propen-1-one] (3PO), a compound able to inhibit the glycolytic flux partially and transiently and to reduce pathological angiogenesis in a variety of disease models. Normal and TNFa induced inflamed ECs were incubated with and without 3PO at a concentration (20 mu M) able to inhibit cell proliferation without cell death. At the end of the incubation period, samples were submitted to the following steps: (a) whole protein extraction, reduction, alkylation, and digestion by trypsin; (b) peptide separation by nano-LC-MS/MS analysis using a high-resolution mass spectrometer; (c) data analysis including protein identification, quantification, and statistical analysis. An altered protein expression profiling in combination with protein network analysis was employed by using a mass spectrometry-based label-free quantification approach to explore the underlying mechanisms of 3PO at cellular level.
机译:已经使用人的内皮细胞(ECS)来监测通过[3-(3-吡啶1)-1-(4-Pyridiny1)-2-propen-1-one-1-one](3po)的诱导的蛋白质变化,一种能够部分且瞬时抑制糖酵解通量,并降低各种疾病模型中的病理血管生成。正常和TNFA诱导发炎的ECS与浓度(20μm)孵育和没有3Po,能够抑制细胞增殖而没有细胞死亡。在孵育期结束时,将样品提交以下步骤:(a)通过胰蛋白酶的全蛋白质提取,还原,烷基化和消化; (b)使用高分辨率质谱仪通过纳米LC-MS / MS分析的肽分离; (c)数据分析,包括蛋白质鉴定,量化和统计分析。通过使用基于质谱的无标记定量方法使用与蛋白质网络分析相结合的改变的蛋白质表达分析,以探讨细胞水平下3PO的潜在机制。

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