Mojsilovic-Petrovic Jelena, Callaghan Debbie, Cui Hong, Dean Clare, Stanimirovic Danica B, Zhang Wandong
Neurobiology Program, Institute for Biological Sciences, National Research Council of Canada, Ottawa, Ontario, Canada.
J Neuroinflammation. 2007 May 2;4:12. doi: 10.1186/1742-2094-4-12.
Neuroinflammation has been implicated in various brain pathologies characterized by hypoxia and ischemia. Astroglia play an important role in the initiation and propagation of hypoxia/ischemia-induced inflammation by secreting inflammatory chemokines that attract neutrophils and monocytes into the brain. However, triggers of chemokine up-regulation by hypoxia/ischemia in these cells are poorly understood. Hypoxia-inducible factor-1 (HIF-1) is a dimeric transcriptional factor consisting of HIF-1alpha and HIF-1beta subunits. HIF-1 binds to HIF-1-binding sites in the target genes and activates their transcription. We have recently shown that hypoxia-induced expression of IL-1beta in astrocytes is mediated by HIF-1alpha. In this study, we demonstrate the role of HIF-1alpha in hypoxia-induced up-regulation of inflammatory chemokines, human monocyte chemoattractant protein-1 (MCP-1/CCL2) and mouse MCP-5 (Ccl12), in human and mouse astrocytes, respectively.
Primary fetal human astrocytes or mouse astrocytes generated from HIF-1alpha+/+ and HIF-1alpha+/- mice were subjected to hypoxia (<2% oxygen) or 125 muM CoCl2 for 4 h and 6 h, respectively. The expression of HIF-1alpha, MCP-1 and MCP-5 was determined by semi-quantitative RT-PCR, western blot or ELISA. The interaction of HIF-1alpha with a HIF-1-binding DNA sequence was examined by EMSA and supershift assay. HIF-1-binding sequence in the promoter of MCP-1 gene was cloned and transcriptional activation of MCP-1 by HIF-1alpha was analyzed by reporter gene assay.
Sequence analyses identified HIF-1-binding sites in the promoters of MCP-1 and MCP-5 genes. Both hypoxia and HIF-1alpha inducer, CoCl2, strongly up-regulated HIF-1alpha expression in astrocytes. Mouse HIF-1alpha+/- astrocytes had lower basal levels of HIF-1alpha and MCP-5 expression. The up-regulation of MCP-5 by hypoxia or CoCl2 in HIF-1alpha+/+ and HIF-1alpha+/- astrocytes was correlated with the levels of HIF-1alpha in cells. Both hypoxia and CoCl2 also up-regulated HIF-1alpha and MCP-1 expression in human astrocytes. EMSA assay demonstrated that HIF-1 activated by either hypoxia or CoCl2 binds to wild-type HIF-1-binding DNA sequence, but not the mutant sequence. Furthermore, reporter gene assay demonstrated that hypoxia markedly activated MCP-1 transcription but not the mutated MCP-1 promoter in transfected astrocytes.
These findings suggest that both MCP-1 and MCP-5 are HIF-1 target genes and that HIF-1alpha is involved in transcriptional induction of these two chemokines in astrocytes by hypoxia.
神经炎症与以缺氧和缺血为特征的各种脑部病变有关。星形胶质细胞通过分泌吸引中性粒细胞和单核细胞进入大脑的炎性趋化因子,在缺氧/缺血诱导的炎症的起始和传播中发挥重要作用。然而,这些细胞中缺氧/缺血导致趋化因子上调的触发因素尚不清楚。缺氧诱导因子-1(HIF-1)是一种由HIF-1α和HIF-1β亚基组成的二聚体转录因子。HIF-1与靶基因中的HIF-1结合位点结合并激活其转录。我们最近发现,星形胶质细胞中缺氧诱导的IL-1β表达由HIF-1α介导。在本研究中,我们分别证明了HIF-1α在人源和鼠源星形胶质细胞中缺氧诱导的炎性趋化因子人单核细胞趋化蛋白-1(MCP-1/CCL2)和小鼠MCP-5(Ccl12)上调中的作用。
分别将来自HIF-1α+/+和HIF-1α+/-小鼠的原代人胎儿星形胶质细胞或小鼠星形胶质细胞置于缺氧(<2%氧气)或125μM氯化钴中,分别处理4小时和6小时。通过半定量RT-PCR、蛋白质免疫印迹或酶联免疫吸附测定法测定HIF-1α、MCP-1和MCP-5的表达。通过电泳迁移率变动分析(EMSA)和超迁移分析检测HIF-1α与HIF-1结合DNA序列的相互作用。克隆MCP-1基因启动子中的HIF-1结合序列,并通过报告基因测定法分析HIF-1α对MCP-1的转录激活作用。
序列分析确定了MCP-1和MCP-5基因启动子中的HIF-1结合位点。缺氧和HIF-1α诱导剂氯化钴均强烈上调星形胶质细胞中HIF-1α的表达。小鼠HIF-1α+/-星形胶质细胞中HIF-1α和MCP-5的基础表达水平较低。缺氧或氯化钴对HIF-1α+/+和HIF-1α+/-星形胶质细胞中MCP-5的上调与细胞中HIF-1α的水平相关。缺氧和氯化钴也上调了人星形胶质细胞中HIF-1α和MCP-1的表达。EMSA分析表明,缺氧或氯化钴激活的HIF-1与野生型HIF-1结合DNA序列结合,但不与突变序列结合。此外,报告基因测定表明,缺氧显著激活了转染星形胶质细胞中MCP-1的转录,但未激活突变的MCP-1启动子。
这些发现表明,MCP-1和MCP-5都是HIF-1的靶基因,并且HIF-1α参与缺氧诱导星形胶质细胞中这两种趋化因子转录的过程。
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