氧化应激对大鼠肺泡巨噬细胞中巨噬细胞炎性蛋白-2基因表达的调控
Regulation of macrophage inflammatory protein-2 gene expression by oxidative stress in rat alveolar macrophages.
作者信息
Shi M M, Chong I, Godleski J J, Paulauskis J D
机构信息
Genomic Pathology Laboratory, Pathology and Experimental Toxicology, Parke-Davis Pharmaceutical Research, Warner-Lambert Company and Department of Pathology, the University of Michigan Medical School, Ann Arbor, MI 48105, USA.
出版信息
Immunology. 1999 Jun;97(2):309-15. doi: 10.1046/j.1365-2567.1999.00798.x.
Chemokines are important mediators in the development of inflammation. Our previous work demonstrated that an oxidative stress can up-regulate mRNA expression of a CC chemokine macrophage inflammatory protein (MIP)-1alpha in rat alveolar macrophages. In the present study, we further investigate whether an oxidative stress can regulate the gene expression of a related CXC chemokine MIP-2, involved in both neutrophil chemotaxis and activation. A rat alveolar macrophage cell line (NR8383) was exposed to 10 microg/ml bacterial lipopolysaccharide (LPS) and MIP-2 mRNA levels dramatically increased after 4 hr of stimulation. This increase by LPS was attenuated by co-treatment with the antioxidants N-acetylcysteine and dimethylsulphoxide, suggesting that the induction of MIP-2 mRNA is mediated via the generation of reactive oxygen species. To assess directly the role of oxidative stress on regulation of MIP-2 mRNA expression, macrophages were exposed to H2O2. MIP-2 mRNA levels had significantly increased after 1 hr exposure to 0.5 mm H2O2, were maximally increased after 4 hr and decreased after 6 hr. Co-treatment of macrophages with the transcriptional inhibitor actinomycin D eliminated the H2O2-induction of MIP-2 mRNA, implicating a role for transcriptional activation in increased expression of MIP-2. Genomic cloning of the rat MIP-2 gene 5'-flanking region has identified a consensus nuclear factor-kappaB (NF-kappaB) binding site. Gel-mobility shift assays revealed NF-kappaB binding to the MIP-2 promoter/enhancer sequence was induced by H2O2. LPS treatment for 4 hr also significantly activated NF-kappaB binding, which could also be attenuated by pretreatment with N-acetylcysteine at the doses that reduced MIP-2 mRNA expression. The half-life of MIP-2 mRNA transcripts was also increased by H2O2 treatment. These observations indicate that MIP-2 gene expression is subject to both transcriptional and post-transcriptional control in response to an H2O2 oxidative stress.
趋化因子是炎症发展过程中的重要介质。我们之前的研究表明,氧化应激可上调大鼠肺泡巨噬细胞中CC趋化因子巨噬细胞炎性蛋白(MIP)-1α的mRNA表达。在本研究中,我们进一步探究氧化应激是否能够调节与中性粒细胞趋化和激活相关的CXC趋化因子MIP-2的基因表达。将大鼠肺泡巨噬细胞系(NR8383)暴露于10μg/ml细菌脂多糖(LPS)中,刺激4小时后MIP-2 mRNA水平显著升高。LPS诱导的这种升高可被抗氧化剂N-乙酰半胱氨酸和二甲基亚砜共同处理所减弱,这表明MIP-2 mRNA的诱导是通过活性氧的产生介导的。为了直接评估氧化应激对MIP-2 mRNA表达调控的作用,将巨噬细胞暴露于H2O2。暴露于0.5 mM H2O2 1小时后MIP-2 mRNA水平显著升高,4小时后达到最大升高,6小时后下降。巨噬细胞与转录抑制剂放线菌素D共同处理消除了H2O2对MIP-2 mRNA的诱导,这表明转录激活在MIP-2表达增加中起作用。大鼠MIP-2基因5'-侧翼区域的基因组克隆鉴定出一个共有核因子-κB(NF-κB)结合位点。凝胶迁移率变动分析显示,H2O2诱导NF-κB与MIP-2启动子/增强子序列结合。LPS处理4小时也显著激活NF-κB结合,这也可被以降低MIP-2 mRNA表达的剂量预先用N-乙酰半胱氨酸处理所减弱。H2O2处理还增加了MIP-2 mRNA转录本的半衰期。这些观察结果表明,响应H2O2氧化应激,MIP-2基因表达受到转录和转录后控制。
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