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Lipopolysaccharide-induced NF-κB nuclear translocation is primarily dependent on MyD88 but TNFα expression requires TRIF and MyD88

机译:脂多糖诱导的NF-κB核易位主要取决于MyD88但TNFα表达需要TRIF和MyD88

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摘要

TLR4 signalling through the MyD88 and TRIF-dependent pathways initiates translocation of the transcription factor NF-κB into the nucleus. In cell population studies using mathematical modeling and functional analyses, Cheng et al. suggested that LPS-driven activation of MyD88, in the absence of TRIF, impairs NF-κB translocation. We tested the model proposed by Cheng et al. using real-time single cell analysis in macrophages expressing EGFP-tagged p65 and a TNFα promoter-driven mCherry. Following LPS stimulation, cells lacking TRIF show a pattern of NF-κB dynamics that is unaltered from wild-type cells, but activation of the TNFα promoter is impaired. In macrophages lacking MyD88, there is minimal NF-κB translocation to the nucleus in response to LPS stimulation, and there is no activation of the TNFα promoter. These findings confirm that signalling through MyD88 is the primary driver for LPS-dependent NF-κB translocation to the nucleus. The pattern of NF-κB dynamics in TRIF-deficient cells does not, however, directly reflect the kinetics of TNFα promoter activation, supporting the concept that TRIF-dependent signalling plays an important role in the transcription of this cytokine.
机译:通过MyD88和TRIF依赖性途径的TLR4信号传导启动了转录因子NF-κB向核内的转运。在使用数学建模和功能分析的细胞群体研究中,Cheng等人。提示在没有TRIF的情况下LPS驱动的MyD88激活会损害NF-κB易位。我们测试了Cheng等人提出的模型。在表达EGFP标签的p65和TNFα启动子驱动的mCherry的巨噬细胞中使用实时单细胞分析。在LPS刺激后,缺乏TRIF的细胞显示出与野生型细胞相同的NF-κB动力学模式,但TNFα启动子的激活受到损害。在缺乏MyD88的巨噬细胞中,响应LPS刺激,NF-κB向细胞核的转运极少,并且TNFα启动子也没有激活。这些发现证实,通过MyD88进行信号传导是LPS依赖性NF-κB易位至细胞核的主要驱动力。但是,TRIF缺陷型细胞中的NF-κB动力学模式并未直接反映TNFα启动子激活的动力学,支持了TRIF依赖性信号在该细胞因子的转录中起重要作用的概念。

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