Pagès G, Stanley E R, Le Gall M, Brunet A, Pouysségur J
Centre de Biochimie, CNRS UMR134, Nice, France.
J Biol Chem. 1995 Nov 10;270(45):26986-92. doi: 10.1074/jbc.270.45.26986.
Mitogen-activated protein kinase (MAPK) or extracellular signal-regulated kinase are ubiquitous kinases conserved from fungi to mammals. Their activity is regulated by phosphorylation on both threonine and tyrosine, and they play a crucial role in the regulation of proliferation and differentiation. We report here the cloning of the murine p44 MAP kinase (extracellular signal-regulated kinase 1) gene, the determination of its intron/exon boundaries, and the characterization of its promoter. The gene spans approximately eight kilobases (kb) and can be divided into nine exons and eight introns, each coding region exon containing from one to three of the highly conserved protein kinase domains. Primer extension analysis reveals the existence of two major start sites of transcription located at -183 and -186 base pairs (bp) as well as four discrete start sites for transcription located at -178, -192, -273, and -292 bp of the initiation of translation. However, the start site region lacks TATA-like sequences but does contain initiator-like sequences proximal to the major start sites obtained by primer extension. 1 kb of the promoter region has been sequenced. It contains three putative TATA boxes far upstream of the main start sites region, one AP-1 box, one AP-2 box, one Malt box, one GAGA box, one half serum-responsive element, and putative binding sites for Sp1 (five), GC-rich binding factor (five), CTF-NF1 (one), Myb (one), p53 (two), Ets-1 (one), NF-IL6 (two), MyoD (two), Zeste (one), and hepatocyte nuclear factor-5 (one). To determine the sites critical for the function of the p44 MAPK promoter, we constructed a series of chimeric genes containing variable regions of the 5'-flanking sequence of p44 MAPK gene and the coding region for luciferase. Activity of the promoter, measured by its capacity to direct expression of a luciferase reporter gene, is strong, being comparable with the activity of the Rous sarcoma virus promoter. Progressive deletions of the approximately 1 kb (-1200/-78) promoter region allowed us to define a minimal region of 186 bp (-284/-78) that has maximal promoter activity. Within this context, deletion of the AP-2 binding site reduces by 30-40% the activity of the promoter. Further deletion of this minimal promoter that removes the major start sites (-167/-78) surprisingly preserves promoter activity. This result implicates a major role of this region that contains the Sp1 sites.(ABSTRACT TRUNCATED AT 400 WORDS)
丝裂原活化蛋白激酶(MAPK)或细胞外信号调节激酶是从真菌到哺乳动物都保守存在的普遍激酶。它们的活性通过苏氨酸和酪氨酸的磷酸化来调节,并且在增殖和分化的调节中起关键作用。我们在此报告小鼠p44 MAP激酶(细胞外信号调节激酶1)基因的克隆、其内含子/外显子边界的确定以及其启动子的特征。该基因跨度约8千碱基(kb),可分为9个外显子和8个内含子,每个编码区外显子包含1至3个高度保守的蛋白激酶结构域。引物延伸分析揭示了位于翻译起始位点-183和-186碱基对(bp)处的两个主要转录起始位点以及位于-178、-192、-273和-292 bp处的四个离散转录起始位点。然而,起始位点区域缺乏TATA样序列,但在引物延伸获得的主要起始位点附近确实含有起始子样序列。已对1 kb的启动子区域进行了测序。它在主要起始位点区域的上游很远位置含有三个推定的TATA盒、一个AP-1盒、一个AP-2盒、一个Malt盒、一个GAGA盒、一个半血清反应元件以及Sp1(五个)、富含GC结合因子(五个)、CTF-NF1(一个)、Myb(一个)、p53(两个)、Ets-1(一个)、NF-IL6(两个)、MyoD(两个)、Zeste(一个)和肝细胞核因子-5(一个)的推定结合位点。为了确定对p44 MAPK启动子功能至关重要的位点,我们构建了一系列嵌合基因,这些基因包含p44 MAPK基因5'侧翼序列的可变区域和荧光素酶的编码区域。通过其指导荧光素酶报告基因表达的能力来测量的启动子活性很强,与劳氏肉瘤病毒启动子的活性相当。对大约1 kb(-1200 / -78)启动子区域进行逐步缺失,使我们能够确定一个186 bp(-284 / -78)的最小区域,该区域具有最大的启动子活性。在此背景下,AP-2结合位点的缺失使启动子活性降低30 - 40%。进一步缺失这个去除主要起始位点(-167 / -78)的最小启动子,令人惊讶地保留了启动子活性。这一结果表明该包含Sp1位点的区域起主要作用。(摘要截短于400字)
