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使用质谱流式细胞术(CyTOF)对细胞因子刺激的外周血单核细胞进行磷酸化流式分析。

Cytokine-stimulated Phosphoflow of PBMC Using CyTOF Mass Cytometry.

作者信息

Fernandez Rosemary, Maecker Holden

机构信息

Human Immune Monitoring Center, Stanford University, Stanford, USA.

出版信息

Bio Protoc. 2015 Jun 5;5(11).

Abstract

Phosphorylation of tyrosine, serine, and threonine residues is critical for the control of protein activity involved in various cellular events. An assortment of kinases and phosphatases regulate intracellular protein phosphorylation in many different cell signaling pathways. These pathways include T and B cell signaling, regulating growth and cell cycle control, plus cytokine, chemokine, and stress responses. Phosphoflow assays combine phosphoprotein-specific antibodies with the power of flow cytometry to enhance phosphoprotein study. In our assay, peripheral blood mononuclear cells are stimulated by cytokines, fixed, surface-stained with a cocktail of antibodies labeled with MAXPAR (brand name) metal-chelating polymers and permeabilized with methanol. They are then stained with intracellular phospho-specific antibodies. We use a CyTOF mass cytometer to acquire the ICP-MS (inductively coupled plasma mass spectrometry) data. The current mass window selected is approximately AW 103-203, which includes the lanthanides used for most antibody labeling, as well as iridium and rhodium for DNA intercalators. Subsequent analysis of the dual count signal data using FlowJo software allows for cell types to be analyzed based on the dual count signal in each mass channel. The percentage of each cell type is determined and reported as a percent of the parent cell type. Median values are reported to quantitate the level of phosphorylation of each protein in response to stimulation. Comparing the level of phosphorylation between samples can offer insight to the status of the immune system.

摘要

酪氨酸、丝氨酸和苏氨酸残基的磷酸化对于控制参与各种细胞事件的蛋白质活性至关重要。各种各样的激酶和磷酸酶在许多不同的细胞信号通路中调节细胞内蛋白质磷酸化。这些通路包括T细胞和B细胞信号传导、调节生长和细胞周期控制,以及细胞因子、趋化因子和应激反应。磷酸化流式细胞术分析将磷酸化蛋白特异性抗体与流式细胞术的强大功能相结合,以加强对磷酸化蛋白的研究。在我们的分析中,外周血单个核细胞受到细胞因子刺激,固定后,用标记有MAXPAR(品牌名)金属螯合聚合物的抗体混合物进行表面染色,并用甲醇进行通透处理。然后用细胞内磷酸化特异性抗体进行染色。我们使用CyTOF质谱流式细胞仪获取电感耦合等离子体质谱(ICP-MS)数据。当前选择的质量窗口约为原子量103 - 203,其中包括用于大多数抗体标记的镧系元素,以及用于DNA嵌入剂的铱和铑。随后使用FlowJo软件对双计数信号数据进行分析,可根据每个质量通道中的双计数信号对细胞类型进行分析。确定每种细胞类型的百分比,并报告为母细胞类型的百分比。报告中位数以定量每种蛋白质在受到刺激后的磷酸化水平。比较样本之间的磷酸化水平可以深入了解免疫系统的状态。

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