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培养的脂肪基质细胞的细胞表面蛋白质组。

The cell-surface proteome of cultured adipose stromal cells.

作者信息

Donnenberg Albert D, Meyer E Michael, Rubin J Peter, Donnenberg Vera S

机构信息

Department of Medicine, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania.

University of Pittsburgh Cancer Institute, Pittsburgh, Pennsylvania.

出版信息

Cytometry A. 2015 Jul;87(7):665-74. doi: 10.1002/cyto.a.22682. Epub 2015 Apr 30.

DOI:10.1002/cyto.a.22682
PMID:25929697
Abstract

In this technical note we describe a method to evaluate the cell surface proteome of human primary cell cultures and cell lines. The method utilizes the BD Biosciences lyoplate, a system covering 242 surface proteins, glycoproteins, and glycosphingolipids plus relevant isotype controls, automated plate-based flow cytometry, conventional file-level analysis and unsupervised K-means clustering of markers on the basis of percent of positive events and mean fluorescence intensity of positive and total clean events. As an example, we determined the cell surface proteome of cultured adipose stromal cells (ASC) derived from 5 independent clinical isolates. Between-sample agreement of very strongly expressed (n = 32) and strongly expressed (n =16) markers was excellent, constituting a reliable profile for ASC identification and determination of functional properties. Known mesenchymal markers (CD29, CD44, CD73, CD90, CD105) were among the identified strongly expressed determinants. Among other strongly expressed markers are several that are potentially immunomodulatory including three proteins that protect from complement mediated effects (CD46, CD55, and CD59), two that regulate apoptosis (CD77 and CD95) and several with ectoenzymatic (CD10, CD26, CD13, CD73, and CD143) or receptor tyrosine kinase (CD140b (PDGFR), CD340 (Her-2), EGFR) activity, suggesting mechanisms for the anti-inflammatory and tissue remodeling properties of ASC. Because variables are standardized for K-means clustering, results generated using this methodology should be comparable between instrumentation platforms. It is widely generalizable to human primary explant cultures and cells lines and will prove useful to determine how cell passage, culture interventions, and gene expression and silencing affect the cell-surface proteome.

摘要

在本技术说明中,我们描述了一种评估人原代细胞培养物和细胞系细胞表面蛋白质组的方法。该方法利用BD Biosciences冻干板,这是一个涵盖242种表面蛋白、糖蛋白和糖鞘脂以及相关同型对照的系统,基于板的自动流式细胞术、传统的文件级分析以及根据阳性事件百分比和阳性及总清洁事件的平均荧光强度对标记物进行无监督K均值聚类。例如,我们确定了源自5个独立临床分离株的培养脂肪基质细胞(ASC)的细胞表面蛋白质组。表达非常强(n = 32)和表达强(n = 16)的标记物在样本间的一致性非常好,构成了用于ASC鉴定和功能特性测定的可靠图谱。已知的间充质标记物(CD29、CD44、CD73、CD90、CD105)是鉴定出的强表达决定因素之一。其他强表达标记物包括几种可能具有免疫调节作用的标记物,其中三种蛋白可保护细胞免受补体介导的效应(CD46、CD55和CD59),两种蛋白调节细胞凋亡(CD77和CD95),还有几种具有外切酶活性(CD10、CD26、CD13、CD73和CD143)或受体酪氨酸激酶活性(CD140b(PDGFR)、CD340(Her-2)、EGFR),这提示了ASC抗炎和组织重塑特性的机制。由于K均值聚类的变量是标准化的,使用该方法生成的结果在不同仪器平台之间应该具有可比性。它可广泛应用于人原代外植体培养物和细胞系,对于确定细胞传代、培养干预以及基因表达和沉默如何影响细胞表面蛋白质组将是有用的。

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