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通过对冯·希佩尔-林道转染细胞系模型进行稳定同位素标记,对肾细胞癌中差异表达的质膜蛋白进行蛋白质组学鉴定。

Proteomic identification of differentially expressed plasma membrane proteins in renal cell carcinoma by stable isotope labelling of a von Hippel-Lindau transfectant cell line model.

作者信息

Aggelis Vassilis, Craven Rachel A, Peng Jianhe, Harnden Patricia, Cairns David A, Maher Eamonn R, Tonge Robert, Selby Peter J, Banks Rosamonde E

机构信息

Cancer Research UK Clinical Centre, St. James's University Hospital, Leeds, UK.

出版信息

Proteomics. 2009 Apr;9(8):2118-30. doi: 10.1002/pmic.200800756.

DOI:10.1002/pmic.200800756
PMID:19337990
Abstract

The von Hippel-Lindau (VHL) tumour suppressor gene plays a central role in development of clear cell renal cell carcinoma (RCC). Using a cell line pair generated from the VHL-defective RCC cell line UMRC2 by transfection with vector control or VHL (-/+VHL) and stable isotope labelling with amino acids in cell culture (SILAC) followed by enrichment of plasma membrane proteins by cell surface biotinylation/avidin-affinity chromatography and analysis by GeLC-MS/MS, VHL-associated changes in plasma membrane proteins were analysed. Comparative analysis of -/+VHL cells identified 19 differentially expressed proteins which were confirmed by reciprocal SILAC labelling. These included several proteins previously reported to be VHL targets, such as transferrin receptor 1 and the alpha 3 and beta1 integrin subunits and novel findings including upregulation of CD166 and CD147 in VHL-defective cells. Western blotting confirmed these changes and also revealed VHL-dependent alterations in protein form for CD147 and CD166, which in the case of CD166 was shown to be due to differential glycosylation. Analysis of patient-matched normal and malignant renal tissues confirmed these differences were also present in vivo in a subset of clear cell RCCs. These results illustrate the potential of this approach for identifying VHL-dependent proteins that may be important in tumorigenesis.

摘要

冯·希佩尔-林道(VHL)肿瘤抑制基因在透明细胞肾细胞癌(RCC)的发展中起着核心作用。通过用载体对照或VHL(-/+VHL)转染,从VHL缺陷型肾癌细胞系UMRC2生成一对细胞系,并在细胞培养中用氨基酸进行稳定同位素标记(SILAC),随后通过细胞表面生物素化/抗生物素蛋白亲和色谱法富集质膜蛋白,并通过GeLC-MS/MS进行分析,从而分析了与VHL相关的质膜蛋白变化。对-/+VHL细胞的比较分析鉴定出19种差异表达的蛋白,这些蛋白通过相互SILAC标记得到了证实。其中包括一些先前报道的VHL靶点蛋白,如转铁蛋白受体1以及α3和β1整合素亚基,还有一些新发现,包括VHL缺陷型细胞中CD166和CD147的上调。蛋白质印迹法证实了这些变化,还揭示了CD147和CD166的蛋白形式存在VHL依赖性改变,就CD166而言,这被证明是由于糖基化差异所致。对患者匹配的正常和恶性肾组织的分析证实,这些差异在一部分透明细胞RCC的体内也存在。这些结果说明了这种方法在鉴定可能在肿瘤发生中起重要作用的VHL依赖性蛋白方面的潜力。

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