Zhang Qian, Wang Hong Y, Liu Xiaobin, Wasik Mariusz A
Department of Pathology and Laboratory Medicine, University of Pennsylvania, 3400 Spruce Street, Philadelphia, Pennsylvania 19104-4283, USA.
Nat Med. 2007 Nov;13(11):1341-8. doi: 10.1038/nm1659. Epub 2007 Oct 7.
Although STAT5A and STAT5B have some nonredundant functional properties, their distinct contributions to carcinogenesis are not clearly defined. Here we report that STAT5A expression is selectively inhibited by DNA methylation of the STAT5A gene promoter region in cells expressing the oncogenic tyrosine kinase NPM1-ALK (also known as NPM-ALK). The DNA methylation is induced by NPM1-ALK itself via STAT3, and is associated with binding to the promoter of the gene encoding MeCP2 capping protein and with lack of binding of the STAT5A gene transcription activator SP1. Reversal of methylation by the DNA methyltransferase inhibitor 5'-aza-2'-deoxycytidine restores SP1 binding and STAT5A gene expression. Notably, the induced or exogenously expressed STAT5A protein binds to the enhancer and intron 14 of the NPM1-ALK gene and triggers selective suppression of NPM1-ALK expression. These results show that NPM1-ALK induces epigenetic silencing of STAT5A gene and that STAT5A protein can act as a key tumor suppressor by reciprocally inhibiting expression of NPM1-ALK.
尽管STAT5A和STAT5B具有一些非冗余的功能特性,但它们对肿瘤发生的不同贡献尚未明确界定。在此我们报告,在表达致癌性酪氨酸激酶NPM1-ALK(也称为NPM-ALK)的细胞中,STAT5A基因启动子区域的DNA甲基化可选择性抑制STAT5A的表达。这种DNA甲基化由NPM1-ALK自身通过STAT3诱导产生,并且与编码MeCP2帽蛋白的基因启动子结合以及STAT5A基因转录激活因子SP1的缺失结合有关。DNA甲基转移酶抑制剂5'-氮杂-2'-脱氧胞苷使甲基化逆转,可恢复SP1结合及STAT5A基因表达。值得注意的是,诱导或外源表达的STAT5A蛋白与NPM1-ALK基因的增强子和内含子14结合,并触发NPM1-ALK表达的选择性抑制。这些结果表明,NPM1-ALK诱导STAT5A基因的表观遗传沉默,并且STAT5A蛋白可通过相互抑制NPM1-ALK的表达而作为关键的肿瘤抑制因子。