人 IRAK-M 的死亡结构域的功能。
The structure function of the death domain of human IRAK-M.
出版信息
Cell Commun Signal. 2014 Dec 7;12:77. doi: 10.1186/s12964-014-0077-3.
BACKGROUND
IRAK-M is an inhibitor of Toll-like receptor signaling that acts by re-directing IRAK-4 activity to TAK1 independent NF-κB activation and by inhibition of IRAK-1/IRAK-2 activity. IRAK-M is expressed in monocytes/macrophages and lung epithelial cells. Lack of IRAK-M in mice greatly improves the resistance to nosocomial pneumonia and lung tumors, which entices IRAK-M as a potential therapeutic target. IRAK-M consists of an N-terminal death domain (DD), a dysfunctional kinase domain and unstructured C-terminal domain. Little is known however on IRAK-M's structure-function relationships.
RESULTS
Since death domains provide the important interactions of IRAK-1, IRAK-2 and IRAK-4 molecules, we generated a 3D structure model of the human IRAK-M-DD (residues C5-G119) to guide mutagenesis studies and predict protein-protein interaction points. First we identified the DD residues involved in the endogenous capacity of IRAK-M to activate NF-κB that is displayed upon overexpression in 293T cells. W74 and R97, at distinct interfaces of the IRAK-M-DD, were crucial for this endogenous NF-κB activating capacity, as well as the C-terminal domain (S445-E596) of IRAK-M. Resulting anti-inflammatory A20 and pro-inflammatory IL-8 transcription in 293T cells was W74 dependent, while IL-8 protein expression was dependent on R97 and the TRAF6 binding motif at P478. The IRAK-M-DD W74 and R97 binding interfaces are predicted to interact with opposite sides of IRAK-4-DD's. Secondly we identified DD residues important for the inhibitory action of IRAK-M by stable overexpression of mutants in THP-1 macrophages and H292 lung epithelial cells. IRAK-M inhibited TLR2/4-mediated cytokine production in macrophages in a manner that is largely dependent on W74. R97 was not involved in inhibition of TNF production but was engaged in IL-6 down-regulation by IRAK-M. Protein-interactive residues D19-A23, located in between W74 and R97, were also observed to be crucial for inhibition of TLR2/4 mediated cytokine induction in macrophages. Remarkably, IRAK-M inhibited TLR5 mediated IL-8 production by lung epithelial cells independent of W74 and R97, but dependent on D19-A23 and R70, two surface-exposed regions that harbor predicted IRAK-2-DD interaction points of IRAK-M.
CONCLUSION
IRAK-M employs alternate residues of its DD to inhibit the different inflammatory mediators induced by varying TLRs and cells.
背景
IRAK-M 是 Toll 样受体信号的抑制剂,通过将 IRAK-4 的活性重新导向 TAK1 非依赖性 NF-κB 激活以及抑制 IRAK-1/IRAK-2 活性来发挥作用。IRAK-M 在单核细胞/巨噬细胞和肺上皮细胞中表达。在小鼠中缺乏 IRAK-M 极大地提高了对医院获得性肺炎和肺肿瘤的抵抗力,这诱使 IRAK-M 成为一个潜在的治疗靶点。IRAK-M 由一个 N 端死亡域(DD)、一个功能失调的激酶域和无结构的 C 端域组成。然而,关于 IRAK-M 的结构-功能关系知之甚少。
结果
由于死亡域提供了 IRAK-1、IRAK-2 和 IRAK-4 分子的重要相互作用,我们生成了人 IRAK-M-DD(残基 C5-G119)的 3D 结构模型,以指导突变研究并预测蛋白质-蛋白质相互作用点。首先,我们确定了 IRAK-M-DD 中参与内源性 IRAK-M 激活 NF-κB 的残基,该激活作用在 293T 细胞中过表达时表现出来。W74 和 R97,位于 IRAK-M-DD 的不同界面上,对于这种内源性 NF-κB 激活能力以及 IRAK-M 的 C 端结构域(S445-E596)至关重要。结果显示,293T 细胞中的抗炎 A20 和促炎 IL-8 转录依赖于 W74,而 IL-8 蛋白表达依赖于 R97 和 P478 处的 TRAF6 结合基序。预测 IRAK-M-DD 的 W74 和 R97 结合界面与 IRAK-4-DD 的相对侧相互作用。其次,我们通过在 THP-1 巨噬细胞和 H292 肺上皮细胞中稳定过表达突变体,确定了 IRAK-M 抑制作用所必需的 DD 残基。IRAK-M 以很大程度上依赖于 W74 的方式抑制 TLR2/4 介导的细胞因子产生。R97 不参与 TNF 产生的抑制,但参与 IRAK-M 下调 IL-6。位于 W74 和 R97 之间的 D19-A23 蛋白相互作用残基也被观察到对巨噬细胞中 TLR2/4 介导的细胞因子诱导的抑制至关重要。值得注意的是,IRAK-M 抑制 TLR5 介导的肺上皮细胞中 IL-8 的产生,这与 W74 和 R97 无关,但依赖于 D19-A23 和 R70,这两个表面暴露区域具有 IRAK-M 的 IRAK-2-DD 相互作用点预测。
结论
IRAK-M 利用其 DD 的替代残基来抑制不同 TLR 和细胞诱导的不同炎症介质。
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