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首页> 外文期刊>Journal of Leukocyte Biology: An Official Publication of the Reticuloendothelial Society >Endotoxin tolerance dysregulates MyD88- and Toll/IL-1R domain-containing adapter inducing IFN-beta-dependent pathways and increases expression of negative regulators of TLR signaling.
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Endotoxin tolerance dysregulates MyD88- and Toll/IL-1R domain-containing adapter inducing IFN-beta-dependent pathways and increases expression of negative regulators of TLR signaling.

机译:内毒素耐受性失调调节MyD88-和Toll / IL-1R结构域的适配器诱导IFN-β依赖性途径,并增加TLR信号转导的负调节剂的表达。

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Endotoxin tolerance reprograms cell responses to LPS by repressing expression of proinflammatory cytokines, while not inhibiting production of anti-inflammatory cytokines and antimicrobial effectors. Molecular mechanisms of induction and maintenance of endotoxin tolerance are incompletely understood, particularly with regard to the impact of endotoxin tolerization on signalosome assembly, activation of adaptor-kinase modules, and expression of negative regulators of TLR signaling in human cells. In this study, we examined LPS-mediated activation of MyD88-dependent and Toll-IL-1R-containing adaptor inducing IFN-beta (TRIF)-dependent pathways emanating from TLR4 and expression of negative regulators of TLR signaling in control and endotoxin-tolerant human monocytes. Endotoxin tolerization suppressed LPS-inducible TLR4-TRIF and TRIF-TANK binding kinase (TBK)1 associations, induction of TBK1 kinase activity, activation of IFN regulatory factor (IRF)-3, and expression of RANTES and IFN-beta. Tolerance-mediated dysregulation of the TLR4-TRIF-TBK1 signaling module was accompanied by increased levels of suppressor of IkappaB kinase-epsilon (SIKE) and sterile alpha and Armadillo motif-containing molecule (SARM). LPS-tolerant cells showed increased expression of negative regulators Toll-interacting protein (Tollip), suppressor of cytokine signaling (SOCS)-1, IL-1R-associated kinase-M, and SHIP-1, which correlated with reduced p38 phosphorylation, IkappaB-alpha degradation, and inhibited expression of TNF-alpha, IL-6, and IL-8. To examine functional consequences of increased expression of Tollip in LPS-tolerized cells, we overexpressed Tollip in 293/TLR4/MD-2 transfectants and observed blunted LPS-inducible activation of NF-kappaB and RANTES, while TNF-alpha responses were not affected. These data demonstrate dysregulation of TLR4-triggered MyD88- and TRIF-dependent signaling pathways and increased expression of negative regulators of TLR signaling in endotoxin-tolerant human monocytes.
机译:内毒素耐受性通过抑制促炎细胞因子的表达来重编程对LPS的细胞应答,同时不抑制抗炎细胞因子和抗菌剂的产生。对内毒素耐受性的诱导和维持的分子机制尚未完全理解,特别是关于内毒素耐受性对信号小体组装,衔接激酶模块的激活以及人类细胞中TLR信号转导的负调控子的表达的影响。在这项研究中,我们检查了LPS介导的MyD88依赖和Toll-IL-1R含衔接子的激活,这些适配器诱导TLR4产生的IFN-β(TRIF)依赖途径以及在对照和内毒素耐受中TLR信号的负调节剂的表达人单核细胞。内毒素耐受性抑制LPS诱导的TLR4-TRIF和TRIF-TANK结合激酶(TBK)1协会,TBK1激酶活性的诱导,IFN调节因子(IRF)-3的激活以及RANTES和IFN-β的表达。耐受介导的TLR4-TRIF-TBK1信号传导模块的失调伴随着IkappaB激酶-ε(SIKE)和无菌α-和含犰狳基序的分子(SARM)抑制剂水平的提高。 LPS耐受细胞显示负调节因子Toll相互作用蛋白(Tollip),细胞因子信号传导抑制因子(SOCS)-1,IL-1R相关激酶M和SHIP-1的表达增加,这与p38磷酸化降低,IkappaB相关-α降解,并抑制TNF-α,IL-6和IL-8的表达。为了检查在LPS耐受的细胞中Tollip表达增加的功能后果,我们在293 / TLR4 / MD-2转染子中过表达Tollip,观察到LPS诱导的NF-kappaB和RANTES激活减弱,而TNF-α反应却不受影响。这些数据证明内毒素耐受的人类单核细胞中TLR4触发的MyD88和TRIF依赖性信号通路的失调和TLR信号负调节剂的表达增加。

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