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从患病组织与正常组织培养的前列腺基质细胞的独特基因表达。

Distinctive gene expression of prostatic stromal cells cultured from diseased versus normal tissues.

作者信息

Zhao Hongjuan, Ramos Cristiane F, Brooks James D, Peehl Donna M

机构信息

Department of Urology, Stanford University, Stanford, California 94305, USA.

出版信息

J Cell Physiol. 2007 Jan;210(1):111-21. doi: 10.1002/jcp.20828.

Abstract

To obtain a comprehensive view of the transcriptional programs in prostatic stromal cells of different histological/pathological origin, we profiled 18 adult human stromal cell cultures from normal transition zone (TZ), normal peripheral zone (PZ), benign prostatic hyperplasia (BPH), and prostate cancer (CA) using cDNA microarrays. A hierarchical clustering analysis of 714 named unique genes whose expression varied at least threefold from the overall mean abundance in at least three samples in all 18 samples demonstrated that cells of different origin displayed distinct gene expression profiles. Many of the differentially expressed genes are involved in biological processes known to be important in the development of prostatic diseases including cell proliferation and apoptosis, cell adhesion, and immune response. Significance Analysis of Microarrays (SAM) analysis identified genes that showed differential expression with statistical significance including 24 genes between cells from TZ versus BPH, 34 between BPH versus CA, and 101 between PZ versus CA. S100A4 and SULF1, the most up- and downregulated genes in BPH versus TZ, respectively, showed expression at the protein level consistent with microarray analysis. In addition, sulfatase assay showed that BPH cells have lower SULF1 activity compared to TZ cells. Quantitative real-time polymerase chain reaction (qRT-PCR) analysis confirmed differential expression of ENPP2/autotoxin and six other genes between PZ versus CA, as well as differential expression of six genes between BPH versus CA. Our results support the hypothesis that prostatic stromal cells of different origin have unique transcriptional programs and point towards genes involved in actions of stromal cells in BPH and CA.

摘要

为全面了解不同组织学/病理学来源的前列腺基质细胞中的转录程序,我们使用cDNA微阵列对来自正常移行区(TZ)、正常外周区(PZ)、良性前列腺增生(BPH)和前列腺癌(CA)的18种成人人类基质细胞培养物进行了分析。对714个命名的独特基因进行层次聚类分析,这些基因在所有18个样本中的至少三个样本中表达变化至少为总体平均丰度的三倍,结果表明不同来源的细胞呈现出不同的基因表达谱。许多差异表达基因参与了已知在前列腺疾病发展中重要的生物学过程,包括细胞增殖和凋亡、细胞粘附以及免疫反应。微阵列显著性分析(SAM)确定了具有统计学差异表达的基因,包括TZ与BPH细胞之间的24个基因、BPH与CA细胞之间的34个基因以及PZ与CA细胞之间的101个基因。S100A4和SULF1分别是BPH与TZ中上调和下调最多的基因,其蛋白水平表达与微阵列分析一致。此外,硫酸酯酶测定表明,与TZ细胞相比,BPH细胞的SULF1活性较低。定量实时聚合酶链反应(qRT-PCR)分析证实了ENPP2/自毒素和其他六个基因在PZ与CA之间的差异表达,以及六个基因在BPH与CA之间的差异表达。我们的结果支持这样的假设,即不同来源的前列腺基质细胞具有独特的转录程序,并指向参与BPH和CA中基质细胞作用的基因。

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