Zhang Xia, Edwards Justin P, Mosser David M
Department of Cell Biology and Molecular Genetics, University of Maryland, College Park, MD 20742, USA.
J Immunol. 2006 Jul 15;177(2):1282-8. doi: 10.4049/jimmunol.177.2.1282.
To gain insight into the molecular mechanism(s) whereby macrophages produce large amounts of IL-10, we analyzed IL-10 gene expression and temporally correlated it with modifications to chromatin associated with the IL-10 promoter. In resting cells, which make essentially no cytokines, the IL-10 promoter is associated with histones containing little or no detectable modifications. Macrophages stimulated in the presence of immune complexes begin to produce high levels of IL-10 pre-mRNA transcripts within minutes of stimulation. Coincident with this transcription was a rapid and dynamic phosphorylation of histone H3 at specific sites in the IL-10 promoter. Histone phosphorylation was closely followed by the binding of transcription factors to the IL-10 promoter. Blocking the activation of ERK prevented histone phosphorylation and transcription factor binding to the IL-10 promoter. In contrast to histone phosphorylation, the peak of histone acetylation at this promoter did not occur until after transcription had peaked. Inhibition of histone deactylase did not alter IL-10 gene expression, suggesting that phosphorylation but not acetylation was the proximal event responsible for IL-10 transcription. Our findings reveal a rapid and well-orchestrated series of events in which ERK activation causes a rapid and transient phosphorylation of histone H3 at specific regions of the IL-10 promoter, resulting in a transient exposure of the IL-10 promoter to the transcription factors that bind there. This exposure is essential for the efficient induction of IL-10 gene expression in macrophages. To our knowledge, this represents a unique way in which the expression of a cytokine gene is regulated in macrophages.
为深入了解巨噬细胞产生大量白细胞介素-10(IL-10)的分子机制,我们分析了IL-10基因表达,并将其与IL-10启动子相关染色质的修饰进行时间关联。在基本不产生细胞因子的静息细胞中,IL-10启动子与几乎没有或无法检测到修饰的组蛋白相关。在免疫复合物存在下刺激的巨噬细胞在刺激后几分钟内开始产生高水平的IL-10前体mRNA转录本。与这种转录同时发生的是IL-10启动子特定位点的组蛋白H3快速且动态的磷酸化。组蛋白磷酸化之后紧接着转录因子与IL-10启动子结合。阻断细胞外信号调节激酶(ERK)的激活可防止组蛋白磷酸化以及转录因子与IL-10启动子结合。与组蛋白磷酸化不同,该启动子处的组蛋白乙酰化峰值直到转录达到峰值后才出现。抑制组蛋白去乙酰化酶并未改变IL-10基因表达,这表明磷酸化而非乙酰化是负责IL-10转录的近端事件。我们的研究结果揭示了一系列快速且精心编排的事件,其中ERK激活导致IL-10启动子特定区域的组蛋白H3快速且短暂的磷酸化,从而使IL-10启动子短暂暴露于结合在那里的转录因子。这种暴露对于巨噬细胞中IL-10基因表达的有效诱导至关重要。据我们所知,这代表了巨噬细胞中细胞因子基因表达调控的一种独特方式。