El Gazzar Mohamed, Yoza Barbara K, Hu Jean Y-Q, Cousart Sue L, McCall Charles E
Department of Internal Medicine, Section of Molecular Medicine, Winston-Salem, North Carolina 27157.
Department of Internal Medicine, Section of Molecular Medicine, Winston-Salem, North Carolina 27157; Department of General Surgery, Wake Forest University School of Medicine, Winston-Salem, North Carolina 27157.
J Biol Chem. 2007 Sep 14;282(37):26857-26864. doi: 10.1074/jbc.M704584200. Epub 2007 Jul 23.
Sustained silencing of potentially autotoxic acute proinflammatory genes like tumor necrosis factor alpha (TNFalpha) occurs in circulating leukocytes following the early phase of severe systemic inflammation. Aspects of this gene reprogramming suggest the involvement of epigenetic processes. We used THP-1 human promonocytes, which mimic gene silencing when rendered endotoxin-tolerant in vitro, to test whether TNFalpha proximal promoter nucleosomes and transcription factors adapt to an activation-specific profile by developing characteristic chromatin-based silencing marks. We found increased TNFalpha mRNA levels in endotoxin-responsive cells that was preceded by dissociation of heterochromatin-binding protein 1alpha, demethylation of nucleosomal histone H3 lysine 9 (H3(Lys(9))), increased phosphorylation of the adjacent serine 10 (H3(Ser(10))), and recruitment of NF-kappaB RelA/p65 to the TNFalpha promoter. In contrast, endotoxin-tolerant cells repressed production of TNFalpha mRNA, retained binding of heterochromatin-binding protein 1alpha, sustained methylation of H3(Lys(9)), reduced phosphorylation of H3(Ser(10)), and showed diminished binding of NF-kappaB RelA/p65 to the TNFalpha promoter. Similar levels of NF-kappaB p50 occurred at the TNFalpha promoter in the basal state, during active transcription, and in the silenced phenotype. RelB, which acts as a repressor of TNFalpha transcription, remained bound to the promoter during silencing. These results support an immunodeficiency paradigm where epigenetic changes at the promoter of acute proinflammatory genes mediate their repression during the late phase of severe systemic inflammation.
在严重全身性炎症的早期阶段之后,循环白细胞中会出现对潜在自毒性急性促炎基因(如肿瘤坏死因子α,TNFα)的持续沉默。这种基因重编程的某些方面表明表观遗传过程参与其中。我们使用THP-1人原单核细胞,其在体外诱导内毒素耐受时会模拟基因沉默,以测试TNFα近端启动子核小体和转录因子是否通过形成基于染色质的特征性沉默标记来适应激活特异性谱。我们发现内毒素反应性细胞中TNFα mRNA水平升高,这之前伴随着异染色质结合蛋白1α的解离、核小体组蛋白H3赖氨酸9(H3(Lys(9)))的去甲基化、相邻丝氨酸10(H3(Ser(10)))磷酸化增加以及NF-κB RelA/p65募集到TNFα启动子。相反,内毒素耐受细胞抑制TNFα mRNA的产生,保留异染色质结合蛋白1α的结合,维持H3(Lys(9))的甲基化,降低H3(Ser(10))的磷酸化,并显示NF-κB RelA/p65与TNFα启动子的结合减少。在基础状态、活跃转录期间和沉默表型中,TNFα启动子处的NF-κB p50水平相似。作为TNFα转录抑制因子的RelB在沉默过程中仍与启动子结合。这些结果支持一种免疫缺陷模式,即急性促炎基因启动子处的表观遗传变化在严重全身性炎症后期介导其抑制。
