Smith Natalie, Browning Claudia A, Duroudier Nathalie, Stewart Ceri, Peel Samantha, Swan Caroline, Hall Ian P, Sayers Ian
Division of Therapeutics & Molecular Medicine, University Hospital of Nottingham, Nottingham, UK.
Respir Res. 2007 Sep 28;8(1):68. doi: 10.1186/1465-9921-8-68.
Airway hyper-responsiveness (AHR) is a key feature of asthma and a causal relationship between airway inflammation and AHR has been identified. The aim of the current study was to clarify the effect of proinflammatory cytokines and asthma medication on primary human airway smooth muscle (ASM) inositol phosphate (IPx) signalling and define the regulatory loci involved.
Primary Human ASM cells were isolated from explants of trachealis muscle from individuals with no history of respiratory disease. The effect of cytokine or asthma medication on histamine or bradykinin induced IPx signalling was assessed by [3H] inositol incorporation. Quantitative Real Time PCR was used to measure mRNA levels of receptors and downstream signalling components. Transcriptional mechanisms were explored using a combination of 5'Rapid Amplification of cDNA Ends (5'RACE) and promoter-reporter techniques.
Treatment of Human ASM cells with IL-13, IFN gamma or salmeterol for 24 hours lead to a modest augmentation of histamine induced IPx responses (144.3 +/- 9.3, 126.4 +/- 7.5 and 117.7 +/- 5.2%, p < 0.05). Similarly, TNFalpha, IFN gamma or salmeterol treatment augmented bradykinin induced IPx responses (127.4 +/- 8.3, 128.0 +/- 8.4 and 111.7 +/- 5.0%, P < 0.05). No treatment significantly influenced sodium fluoride induced IPx responses suggesting regulation occurs at the receptor locus. Analyses of mRNA expression of components of the IPx pathway i.e. H1 Histamine Receptor (HRH1), B2 Bradykinin Receptor (BDKRB2), G alpha q/11 and PLC-beta1 identified that a significant induction of receptor mRNA (>2 fold) was a feature of these responses explaining the cytokine and spasmogen specificity. The HRH1 and BDKRB2 promoter regions were mapped in ASM and promoter-reporter analyses identified that salmeterol can induce HRH1 (>2 fold) and BDKRB2 (2-5 fold) transcription. The effect of cytokines on HRH1 and BDKRB2 promoter-reporter expression suggested a more complex regulation of mRNA expression involving additional loci to the core promoter.
Our results indicate that the spasmogen specific receptor locus may be a key site of regulation determining the magnitude of spasmogen mediated ASM IPx responses during airway inflammation or following asthma medication. These data provide further insight into the molecular basis of AHR and extend our understanding of potentially detrimental effects associated with existing therapies used in the treatment of asthma.
气道高反应性(AHR)是哮喘的一个关键特征,并且已经确定气道炎症与AHR之间存在因果关系。本研究的目的是阐明促炎细胞因子和哮喘药物对原代人气道平滑肌(ASM)肌醇磷酸(IPx)信号传导的影响,并确定其中涉及的调控位点。
从无呼吸系统疾病病史个体的气管肌外植体中分离出原代人ASM细胞。通过[3H]肌醇掺入评估细胞因子或哮喘药物对组胺或缓激肽诱导的IPx信号传导的影响。使用定量实时PCR测量受体和下游信号传导成分的mRNA水平。结合5' cDNA末端快速扩增(5'RACE)和启动子报告技术探索转录机制。
用IL-13、IFN-γ或沙美特罗处理人ASM细胞24小时导致组胺诱导的IPx反应适度增强(分别为144.3±9.3%、126.4±7.5%和117.7±5.2%,p<0.05)。同样,TNF-α、IFN-γ或沙美特罗处理增强了缓激肽诱导的IPx反应(分别为127.4±8.3%、128.0±8.4%和111.7±5.0%,P<0.05)。没有处理显著影响氟化钠诱导的IPx反应,表明调节发生在受体位点。对IPx途径成分即H1组胺受体(HRH1)、B2缓激肽受体(BDKRB2)、Gαq/11和PLC-β1的mRNA表达分析表明,受体mRNA的显著诱导(>2倍)是这些反应的一个特征,解释了细胞因子和致痉剂的特异性。在ASM中绘制了HRH1和BDKRB2启动子区域,启动子报告分析确定沙美特罗可诱导HRH1(>2倍)和BDKRB2(2-5倍)转录。细胞因子对HRH1和BDKRB2启动子报告表达的影响表明,mRNA表达的调节更为复杂,涉及核心启动子以外的其他位点。
我们的结果表明,致痉剂特异性受体位点可能是调节的关键位点,决定气道炎症期间或哮喘药物治疗后致痉剂介导的ASM IPx反应的幅度。这些数据进一步深入了解了AHR的分子基础,并扩展了我们对哮喘治疗中现有疗法相关潜在有害影响的理解。
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