Department of Pharmacology, Toxicology, and Experimental Therapeutics, University of Kansas Medical Center, Kansas City, KS 66160, USA.
Liver Int. 2011 Feb;31(2):230-44. doi: 10.1111/j.1478-3231.2010.02347.x. Epub 2010 Sep 29.
BACKGROUND/AIMS: Several studies have shown that regions of hypoxia develop in the liver during chronic injury. Furthermore, it has been demonstrated that hypoxia stimulates the release of mediators from hepatic stellate cells (HSCs) that may affect the progression of fibrosis. The mechanism by which hypoxia modulates gene expression in HSCs is not known. Recent studies demonstrated that the hypoxia-activated transcription factor, hypoxia-inducible factor (HIF)-1α, is critical for the development of fibrosis. Accordingly, the hypothesis was tested that HIF-1α is activated in HSCs and regulates the expression of genes important for HSC activation and liver fibrosis.
Hepatic stellate cells were isolated from mice and exposed to hypoxia. HIF-1α and HIF-2α activation were measured, and gene expression was analysed by gene array analysis. To identify the genes regulated by HIF-1α, HSCs were isolated from control and HIF-1α-deficient mice.
Exposure of primary mouse HSCs to 0.5% oxygen activated HIF-1α and HIF-2α. mRNA levels of numerous genes were increased in HSCs exposed to 0.5% oxygen, many of which are important for HSC function, angiogenesis and collagen synthesis. Of the mRNAs increased, chemokine receptor (Ccr) 1, Ccr5, macrophage migration inhibitory factor, interleukin-13 receptor α1 and prolyl-4-hydroxylase α2 (P4h α2) were completely HIF-1α dependent. Upregulation of the vascular endothelial growth factor and the placental growth factor was partially HIF-1α dependent and upregulation of angiopoietin-like 4 and P4h α1 was HIF-1α independent.
Results from these studies demonstrate that hypoxia, through activation of HIF-1α, regulates the expression of genes that may alter the sensitivity of HSCs to certain activators and chemotaxins, and regulates the expression of genes important for angiogenesis and collagen synthesis.
背景/目的:多项研究表明,慢性损伤过程中肝脏会出现缺氧区域。此外,已有研究表明,缺氧会刺激肝星状细胞(HSCs)释放介质,从而可能影响纤维化的进展。目前尚不清楚缺氧调节 HSCs 基因表达的机制。最近的研究表明,缺氧激活转录因子缺氧诱导因子(HIF)-1α对于纤维化的发展至关重要。因此,我们提出假设,即 HIF-1α在 HSCs 中被激活,并调节与 HSCs 激活和肝纤维化相关的重要基因的表达。
从小鼠中分离肝星状细胞并使其暴露于缺氧环境中。通过基因芯片分析检测 HIF-1α 和 HIF-2α 的激活情况以及基因表达情况。为了鉴定受 HIF-1α 调控的基因,从小鼠中分离出对照组和 HIF-1α 缺陷型 HSCs。
将原代小鼠 HSCs 暴露于 0.5%的氧气中可激活 HIF-1α 和 HIF-2α。在 0.5%氧气环境中培养的 HSCs 中,许多与 HSCs 功能、血管生成和胶原合成相关的基因的 mRNA 水平升高。在这些上调的 mRNA 中,趋化因子受体(Ccr)1、Ccr5、巨噬细胞移动抑制因子、白细胞介素 13 受体 α1 和脯氨酰-4-羟化酶α2(P4hα2)完全依赖于 HIF-1α。血管内皮生长因子和胎盘生长因子的上调部分依赖于 HIF-1α,而血管生成素样 4 和 P4hα1 的上调则与 HIF-1α 无关。
这些研究结果表明,缺氧通过激活 HIF-1α,调节基因的表达,从而改变 HSCs 对某些激活剂和趋化因子的敏感性,并调节与血管生成和胶原合成相关的重要基因的表达。