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小鼠前列腺素E受体亚型EP2基因的特性:巨噬细胞和子宫中转录的组织特异性起始

Characterization of the gene for the mouse prostaglandin E receptor subtype EP2: tissue-specific initiation of transcription in the macrophage and the uterus.

作者信息

Katsuyama M, Sugimoto Y, Okano K, Segi E, Ikegami R, Negishi M, Ichikawa A

机构信息

Department of Physiological Chemistry, Faculty of Pharmaceutical Sciences, Kyoto University, Kyoto 606, Japan.

出版信息

Biochem J. 1998 Mar 15;330 ( Pt 3)(Pt 3):1115-21. doi: 10.1042/bj3301115.

Abstract

Genomic DNA clones for the mouse prostaglandin (PG) E receptor subtype EP2 were isolated and characterized. The mouse EP2 gene is composed of 2 exons and 1 intron, and spans 16 kb. The intron which is approx. 12 kb in length is located at the end of the sixth transmembrane domain, as with other prostanoid receptor genes. Based on this structure, transcripts were analysed in endotoxin-treated macrophages and pseudopregnant uteri, in which abundant expression of EP2 mRNA was observed. Sequence analysis of cDNA clones from these origins and Northern hybridization of these RNAs revealed that the uterine EP2 mRNA (U-type) has a longer 5'-untranslated region than the macrophage EP2 transcript (M-type). The major transcription initiation sites for M-type and U-type EP2 are located 124 and 769 bp upstream of the translation start site, respectively. The M-type was expressed in various tissues, whereas the U-type was found only in the uterus. The 2 kb segment containing the immediate 5'-flanking and 5'-noncoding regions contain three consensus sequences for the NF-IL6 binding site, one consensus sequence for the NF-kappaB binding site, four AP-2 consensus sequences, one AP-4 consensus sequence, one potential cAMP response element, and one potential progesterone response element. These results suggest that EP2 gene expression in the macrophage and uterus is under the control of distinct mechanisms involving alternative promoters.

摘要

分离并鉴定了小鼠前列腺素(PG)E受体亚型EP2的基因组DNA克隆。小鼠EP2基因由2个外显子和1个内含子组成,跨度为16 kb。与其他前列腺素受体基因一样,该内含子长度约为12 kb,位于第六个跨膜结构域的末端。基于这种结构,在内毒素处理的巨噬细胞和假孕子宫中分析了转录本,在这些组织中观察到了EP2 mRNA的丰富表达。对来自这些来源的cDNA克隆进行序列分析以及对这些RNA进行Northern杂交分析表明,子宫EP2 mRNA(U型)的5'-非翻译区比巨噬细胞EP2转录本(M型)更长。M型和U型EP2的主要转录起始位点分别位于翻译起始位点上游124和769 bp处。M型在各种组织中表达,而U型仅在子宫中发现。包含紧邻5'-侧翼和5'-非编码区的2 kb片段含有三个NF-IL6结合位点的共有序列、一个NF-κB结合位点的共有序列、四个AP-2共有序列、一个AP-4共有序列、一个潜在的cAMP反应元件和一个潜在的孕酮反应元件。这些结果表明,巨噬细胞和子宫中EP2基因的表达受涉及替代启动子的不同机制的控制。

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