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白细胞介素-6通过特定的启动子元件下调NTPDase2的转录。

IL-6 downregulates transcription of NTPDase2 via specific promoter elements.

作者信息

Yu Jin, Lavoie Elise G, Sheung Nina, Tremblay Jacques J, Sévigny Jean, Dranoff Jonathan A

机构信息

Yale University School of Medicine, Yale Liver Center, New Haven, CT 06515, USA.

出版信息

Am J Physiol Gastrointest Liver Physiol. 2008 Mar;294(3):G748-56. doi: 10.1152/ajpgi.00208.2007. Epub 2008 Jan 17.

Abstract

Bile ductular proliferation is markedly upregulated in biliary fibrosis and cirrhosis. However, the mechanisms regulating this upregulation in bile ductular proliferation have not been defined. Recently, we demonstrated that expression of the ectonucleotidase nucleoside triphosphate diphosphohydrolase-2 (NTPDase2/Entpd2) by portal fibroblasts (PF) is a critical regulator of bile ductular proliferation. Since interleukin 6 (IL-6) is markedly upregulated in biliary cirrhosis, our aims were to determine the role and mechanism of IL-6 in the regulation of NTPDase2 by PF. We found that IL-6 downregulated NTPDase2 protein expression in a concentration-dependent and time-dependent fashion but did not alter PF alpha-smooth muscle actin expression. IL-6 markedly downregulated NTPDase2 mRNA expression. Expression of the IL-6 receptor gp130 but not the IL-6 receptor gp80 was detected in PF. Two transcription start sites were identified in rat Entpd2 by the method of RNA ligase-mediated rapid amplification of 5' cDNA ends. The minimal promoter construct, but not shorter constructs, was downregulated by IL-6. Three putative IL-6 response elements were identified in silico and mutated. Mutation of all three response elements, but not fewer elements, completely abolished the IL-6 response. Thus IL-6 transcriptionally downregulates NTPDase2 expression by PF via actions at specific promoter elements independently of myofibroblastic differentiation. This effect may represent a novel signaling pathway by which bile ductular proliferation is dysregulated in biliary cirrhosis and thus provides a potential therapeutic approach for the regulation of bile ductular growth.

摘要

胆管增生在胆汁性肝纤维化和肝硬化中显著上调。然而,调节胆管增生上调的机制尚未明确。最近,我们证明了门静脉成纤维细胞(PF)中外核苷酸酶核苷三磷酸二磷酸水解酶-2(NTPDase2/Entpd2)的表达是胆管增生的关键调节因子。由于白细胞介素6(IL-6)在胆汁性肝硬化中显著上调,我们的目的是确定IL-6在PF调节NTPDase2中的作用和机制。我们发现IL-6以浓度和时间依赖性方式下调NTPDase2蛋白表达,但不改变PFα-平滑肌肌动蛋白表达。IL-6显著下调NTPDase2 mRNA表达。在PF中检测到IL-6受体gp130的表达,但未检测到IL-6受体gp80的表达。通过RNA连接酶介导的5' cDNA末端快速扩增方法在大鼠Entpd2中鉴定出两个转录起始位点。最小启动子构建体而非较短的构建体被IL-6下调。通过计算机分析鉴定出三个推定的IL-6反应元件并进行了突变。所有三个反应元件的突变而非较少元件的突变完全消除了IL-6反应。因此,IL-6通过作用于特定启动子元件转录下调PF中NTPDase2的表达,而与肌成纤维细胞分化无关。这种效应可能代表了一种新的信号通路,通过该通路胆汁性肝硬化中胆管增生失调,从而为调节胆管生长提供了一种潜在的治疗方法。

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