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首页> 外文期刊>Surgery >Clathrin heavy chain is required for TNF-induced inflammatory signaling.
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Clathrin heavy chain is required for TNF-induced inflammatory signaling.

机译:网格蛋白重链是TNF诱导的炎症信号传导所必需的。

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BACKGROUND: Tumor necrosis factor receptor I recruits tumor necrosis factor receptor-associated death domain (TRADD) and multiple kinases that ultimately phosphorylate inhibitor kappa B (IKB alpha). Degradation of phospho-IKB alpha (p-IKB alpha) frees nuclear factor kappa B (NFKB) to be active and phosphorylated. Many receptors require clathrin-mediated endocytosis to provide the scaffolds necessary for signaling. Therefore, we investigated the role of clathrin heavy chain (CHC) in tumor necrosis factor alpha (TNF-alpha)-induced IKB alpha phosphorylation and NFKB activation. We hypothesized that CHC was required for TNF-alpha-induced inflammatory signaling. METHODS: We treated human pulmonary epithelial cells with small interfering RNA to knock down intracellular CHC (CHCsil). TRADD and scrambled (noncoding) small interfering RNA sequences were used as positive and negative controls, respectively. Treatment groups were exposed to 10 ng/mL of TNF-alpha. Total I kappaB alpha, p-I kappaB alpha, and phosphorylated P65 (a subunit of NFKB) were determined by immunoblot staining. Densitometry was normalized to controls for the analysis of the stains. TNF-alpha-induced release of monocyte chemoattractant protein 1 (MCP-1) was determined by enzyme-linked immunosorbent assay. Statistical analyses were determined by analysis of variance or paired t test as appropriate. RESULTS: TNF-alpha-induced I kappaB alpha phosphorylation and degradation at 5 and 30 minutes, respectively, and induced P65 phosphorylation. CHCsil diminished p-I kappaB alpha by 91% (P < .03); however, I kappaB alpha degradation was not affected. CHC knockdown caused a 66% decrease in P65 phosphorylation after 3 minutes of TNF-alpha. CHCsil decreased TNF-alpha-induced MCP-1 by 46% (P < .05), compared with control. CONCLUSIONS: CHCsil significantly impairs phosphorylation of both I kappaB alpha and P65. CHCsil also significantly decreased MCP-1 production. These data suggest that CHC is required for certain TNF-alpha-induced, inflammatory signaling pathways.
机译:背景:肿瘤坏死因子受体I募集肿瘤坏死因子受体相关的死亡域(TRADD)和多种激酶,这些激酶最终会磷酸化抑制剂kappa B(IKB alpha)。磷酸化IKBα(p-IKB alpha)的降解释放了核因子kappa B(NFKB),使其具有活性并被磷酸化。许多受体需要网格蛋白介导的内吞作用以提供信号转导所必需的支架。因此,我们研究了网格蛋白重链(CHC)在肿瘤坏死因子α(TNF-α)诱导的IKBα磷酸化和NFKB激活中的作用。我们假设CHC是TNF-α诱导的炎症信号传导所必需的。方法:我们用小的干扰RNA处理人肺上皮细胞,以敲低细胞内CHC(CHCsil)。 TRADD和加扰的(非编码)小干扰RNA序列分别用作阳性和阴性对照。治疗组暴露于10 ng / mL的TNF-α。通过免疫印迹染色确定总的IκBα,pIκBα和磷酸化的P65(NFKB的亚基)。将光密度测定法标准化为对照用于污渍分析。通过酶联免疫吸附试验确定了TNF-α诱导的单核细胞趋化蛋白1(MCP-1)的释放。统计分析通过方差分析或成对t检验确定。结果:TNF-α诱导的I kappaBα磷酸化和降解分别在5和30分钟,并诱导P65磷酸化。 CHCsil使p-I kappaBα降低了91%(P <.03);但是,我kappaB alpha的降解不受影响。 CHC敲低导致TNF-α3分钟后P65磷酸化降低66%。与对照相比,CHCsil使TNF-α诱导的MCP-1降低46%(P <.05)。结论:CHCsil显着损害IκBα和P65的磷酸化。 CHCsil还大大降低了MCP-1的产量。这些数据表明,某些TNF-α诱导的炎症信号通路需要CHC。

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