Rökaeus A, Waschek J A
Department of Medical Biochemistry and Biophysics, Medical Nobel Institute, Karolinska Institutet, Stockholm, Sweden.
DNA Cell Biol. 1994 Aug;13(8):845-55. doi: 10.1089/dna.1994.13.845.
Galanin (GAL) is a biologically active neuropeptide that has been suggested to play a role in stress-induced inhibition of insulin secretion, in dementia of the Alzheimer's type, and in the regulation of growth hormone secretion. We report here the isolation of a bovine genomic clone containing more than 5-kb 5'-flanking sequences. Partial sequence analysis of the genomic clone revealed an atypical TATA-box in the promoter (ATAAATA) and several consensus sequences that typically bind transcription factors, including those that bind NF kappa B, Sp1, and AP-2. Primer extension and RNase protection analyses revealed that transcription is initiated at two sites, 28 and 31 bp, respectively, downstream from the TATA-box. To locate functionally active regulatory elements on the GAL gene, we first identified a neural crest-derived human neuroblastoma cell line, SK-N-SH subclone SH-SY5Y, that expressed easily detectable levels of endogenous GAL mRNA. We then constructed plasmids containing various lengths of bovine GAL 5'-flanking sequences and the first exon fused to a reporter plasmid encoding luciferase. Transfection of these plasmids into the SH-SY5Y cells and analysis by transient expression indicated that 131 bp of 5' gene sequence was sufficient to obtain maximal basal expression. Further, expression was suppressed 16-fold when 5 kb were included, suggesting the presence of a distal repressor element(s). In another set of experiments, we found that GAL mRNA levels could be induced more than 10-fold by 20-hr treatment with phorbol 12-myristate 13-acetate (PMA). In cells transfected with the same plasmids, luciferase activity was also induced by PMA, but the degree of induction did not significantly differ among the deletion constructions (varying from six- to eight-fold), suggesting that elements conferring PMA induction and/or RNA stabilization may be located within 131 bp of the transcriptional start site, in the first exon, or on gene sequences not studied here.
甘丙肽(GAL)是一种生物活性神经肽,有人认为它在应激诱导的胰岛素分泌抑制、阿尔茨海默病型痴呆以及生长激素分泌调节中发挥作用。我们在此报告分离出一个包含超过5kb 5'侧翼序列的牛基因组克隆。对该基因组克隆的部分序列分析揭示了启动子中的一个非典型TATA盒(ATAAATA)以及几个通常结合转录因子的共有序列,包括那些结合核因子κB、Sp1和AP-2的序列。引物延伸和核糖核酸酶保护分析表明转录分别在TATA盒下游28bp和31bp的两个位点起始。为了定位GAL基因上功能活跃的调控元件,我们首先鉴定了一种源自神经嵴的人神经母细胞瘤细胞系,SK-N-SH亚克隆SH-SY5Y,它表达易于检测水平的内源性GAL mRNA。然后我们构建了含有不同长度牛GAL 5'侧翼序列以及与编码荧光素酶的报告质粒融合的第一个外显子的质粒。将这些质粒转染到SH-SY5Y细胞中并通过瞬时表达进行分析,结果表明5'基因序列的131bp足以获得最大基础表达。此外,当包含5kb时表达被抑制了16倍,这表明存在一个远端抑制元件。在另一组实验中,我们发现用佛波酯12-肉豆蔻酸酯13-乙酸酯(PMA)处理20小时可使GAL mRNA水平诱导超过10倍。在用相同质粒转染的细胞中,荧光素酶活性也被PMA诱导,但诱导程度在缺失构建体之间没有显著差异(从6倍到8倍不等),这表明赋予PMA诱导和/或RNA稳定作用的元件可能位于转录起始位点的131bp内、第一个外显子中或此处未研究的基因序列上。
