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首页> 外文期刊>The Biochemical Journal >Sequence of the 5 '-flanking region and promoter activity of the human mucin gene MUC5B in different phenotypes of colon cancer cells
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Sequence of the 5 '-flanking region and promoter activity of the human mucin gene MUC5B in different phenotypes of colon cancer cells

机译:人黏蛋白基因MUC5B 5'侧翼区序列和启动子活性在结肠癌细胞不同表型中的作用

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摘要

Control of gene expression in intestinal cells is poorly understood. Molecular mechanisms that regulate transcription of cellular genes are the foundation for understanding developmental and differentiation events. Mucin gene expression has been shown to be altered in many intestinal diseases and especially cancers of the gastrointestinal tract. Towards understanding the transcriptional regulation of a member of the 11p15.5 human mucin gene cluster, we have characterized 3.55 kb of the 5'-flanking region of the human mucin gene MUC5B, including the promoter, the first two exons and the first intron. We report here the promoter activity of successively 5'-truncated sections of 956 bases of this region by fusing it to the coding region of a luciferase reporter gene. The transcription start site was determined by primer-extension analysis. The region upstream of the transcription start site is characterized by the presence of a TATA box at bases -32/-26, DNA-binding elements for transcription factors c-Myc, N-Myc, Spl and nuclear factor kappa B as well as putative activator protein (AP)-1-, cAMP-response-element-binding protein (CREB)-, hepatocyte nuclear factor (HNF)-1-, HNF-3-, TGT3-, gut-enriched Kruppel factor (GKLF)-, thyroid transcription factor (FTF)-1- and glucocorticoid receptor element (GRE)-binding sites. Intron 1 of MUC5R was also characterized, it is 2511 nucleotides long and contains a DNA segment of 259 bp in which are clustered eight tandemly repeated GA boxes and a CACCC box that bind Sp1. AP-2 alpha and GATA-1 nuclear factors were also shown to bind to their respective cognate elements in intron 1. In transfection studies the MUC5B promoter showed a cell-specific activity as it is very active in mucus-secreting LS174T cells, whereas it is inactive in Caco-2 enterocytes and MT-29 STD (standard) undifferentiated cells. Within the promoter, maximal transcription activity was found in a segment covering the first 223 bp upstream of the transcription start site. Finally, in co-transfection experiments a transactivating effect of Spl on to MUC5B promoter was seen in LS174T and Caco-2 cells. [References: 37]
机译:对肠道细胞中基因表达的控制了解甚少。调节细胞基因转录的分子机制是理解发育和分化事件的基础。已经显示粘蛋白基因表达在许多肠道疾病,尤其是胃肠道癌症中改变。为了理解11p15.5人类粘蛋白基因簇成员的转录调控,我们鉴定了3.55 kb人类粘蛋白基因MUC5B的5'侧翼区域,包括启动子,前两个外显子和第一个内含子。我们在这里报告该区域的956个碱基的5'截短部分的启动子活性,方法是将其融合到荧光素酶报道基因的编码区域。通过引物延伸分析确定转录起始位点。转录起始位点上游区域的特征是在-32 / -26处存在TATA框,转录因子c-Myc,N-Myc,Spl和核因子κB以及推定的DNA结合元件激活蛋白(AP)-1-,cAMP-反应元件结合蛋白(CREB)-,肝细胞核因子(HNF)-1-,HNF-3-,TGT3-,富含肠道的Kruppel因子(GKLF)-,甲状腺转录因子(FTF)-1-和糖皮质激素受体元件(GRE)结合位点。 MUC5R的内含子1的特征还在于,它的长度为2511个核苷酸,并包含259 bp的DNA片段,其中聚集了八个串联重复的GA框和与Sp1结合的CACCC框。还显示了AP-2α和GATA-1核因子与内含子1各自的同源元件结合。在转染研究中,MUC5B启动子显示出细胞特异性活性,因为它在分泌粘液的LS174T细胞中非常活跃,而在Caco-2肠上皮细胞和MT-29 STD(标准)未分化细胞中无活性。在启动子内,在覆盖转录起始位点上游第一个223 bp的片段中发现了最大的转录活性。最后,在共转染实验中,在LS174T和Caco-2细胞中发现了Spl对MUC5B启动子的反式激活作用。 [参考:37]

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