Enya Kazuaki, Hayashi Hidetoshi, Takii Takemasa, Ohoka Nobumichi, Kanata Shinya, Okamoto Takashi, Onozaki Kikuo
Department of Molecular Health Sciences, Graduate School of Pharmaceutical Sciences, Nagoya City University, 3-1 Tanabe-dori, Mizuho-ku, Nagoya, Aichi 467-8603, Japan.
J Leukoc Biol. 2008 Jan;83(1):190-9. doi: 10.1189/jlb.0106008. Epub 2007 Sep 28.
A375-6 human melanoma cells are sensitive to the antiproliferative effect of IL-1. After a long period of culturing, we have obtained cells resistant to IL-1. The resistant clone A375-R8 constitutively produced IL-1 alpha. In this study, we identified a sequence, CGCC, located at -48 to -45 upstream of the transcription start site, to be essential for the constitutive IL-1 alpha gene activation. Specificity protein 1 (Sp1) and Sp3 bound to the nucleotide containing the sequence. Although the binding level to the nucleotide and expression level of Sp1 and Sp3 are comparable in A375-R8 and A375-6 cells, transactivation activity of Sp1 is higher in A375-R8 cells as compared with A375-6 cells. Sp3 could not transactivate the IL-1 alpha promoter. These results suggest that Sp1 but not Sp3 is important for IL-1 alpha gene activation. Trichostatin A (TSA), an inhibitor of histone deacetylase (HDAC), greatly augmented the IL-1 alpha promoter activity in A375-6 cells to the level comparable with that in A375-R8 cells. TSA also induced IL-1 alpha mRNA expression in A375-6 cells. Sp1 and Sp3 bound to HDAC1 in A375-R8 and A375-6 cells. The chromatin immunoprecipitation assay revealed the binding of Sp1 and HDAC1 to the promoter region of the IL-1 alpha gene. The activities of HDAC bound to Sp1 and Sp3, and that of HDAC1 was lower in A375-R8 cells as compared with A375-6 cells. These results indicate that the reduction in the activity and interaction of HDAC1 with Sp1 are critical for the constitutive IL-1 alpha gene expression.
A375 - 6人黑色素瘤细胞对白细胞介素 - 1(IL - 1)的抗增殖作用敏感。经过长时间培养,我们获得了对IL - 1耐药的细胞。耐药克隆A375 - R8组成性地产生IL - 1α。在本研究中,我们确定了位于转录起始位点上游 - 48至 - 45处的序列CGCC对于组成性IL - 1α基因激活至关重要。特异性蛋白1(Sp1)和Sp3与包含该序列的核苷酸结合。尽管在A375 - R8和A375 - 6细胞中,Sp1和Sp3与核苷酸的结合水平以及它们的表达水平相当,但与A375 - 6细胞相比,A375 - R8细胞中Sp1的反式激活活性更高。Sp3不能反式激活IL - 1α启动子。这些结果表明,对于IL - 1α基因激活而言,Sp1而非Sp3很重要。曲古抑菌素A(TSA)是一种组蛋白去乙酰化酶(HDAC)抑制剂,它极大地增强了A375 - 6细胞中IL - 1α启动子活性,使其达到与A375 - R8细胞相当的水平。TSA还诱导了A375 - 6细胞中IL - 1α mRNA的表达。在A375 - R8和A375 - 6细胞中,Sp1和Sp3与HDAC1结合。染色质免疫沉淀分析揭示了Sp1和HDAC1与IL - 1α基因启动子区域的结合。与A375 - 6细胞相比,A375 - R8细胞中与Sp1和Sp3结合的HDAC以及HDAC1的活性较低。这些结果表明,HDAC1活性的降低及其与Sp1相互作用的减弱对于组成性IL - 1α基因表达至关重要。