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UDP-N-乙酰-α-D-半乳糖胺:多肽N-乙酰半乳糖胺基转移酶-3基因在腺癌细胞中表达调控的结构基础

Structural basis for the regulation of UDP-N-acetyl-alpha-D-galactosamine: polypeptide N-acetylgalactosaminyl transferase-3 gene expression in adenocarcinoma cells.

作者信息

Nomoto M, Izumi H, Ise T, Kato K, Takano H, Nagatani G, Shibao K, Ohta R, Imamura T, Kuwano M, Matsuo K, Yamada Y, Itoh H, Kohno K

机构信息

Department of Molecular Biology, University of Occupational and Environmental Health, Japan, School of Medicine, Kitakyushu.

出版信息

Cancer Res. 1999 Dec 15;59(24):6214-22.

Abstract

The UDP-N-acetyl-alpha-D-galactosamine: polypeptide N-acetylgalactosaminyl transferase-3 (Gal NAc-T3) gene, a member of the Gal NAc transferase gene family, is expressed in a tissue-specific manner. To elucidate the function of this gene, we have focused on the molecular mechanism underlying regulation of gene expression. We have cloned Gal NAc-T3 cDNA and used it to show that Gal NAc-T3 mRNA is expressed in tumor cell lines derived from secretory epithelial tissue adenocarcinomas but not in cell lines derived from bladder and epidermoid carcinomas. Using a polyclonal antibody to Gal NAc-T3, we observed protein expression in adenocarcinoma but not non-adenocarcinoma cell lines, and in breast carcinoma cells but not in normal breast tissue. We used Gal NAc-T3 cDNA to isolate three overlapping genomic clones containing the 5'-portion of the human Gal NAc-T3 gene, and we sequenced 1.6 kb around the first exon. A transient expression assay using the luciferase gene showed that promoter activity was much higher in MCF-7 cells than in KB cells. In vivo footprint experiments showed significant protection of a distal GC box, an NRF-1 site, and an AP-2 site in MCF-7 cells. A novel stem and loop structure extending from nucleotide -103 to nucleotide -165 and contiguous to these transcription factor binding sites seemed to be functional in regulating Gal NAc-T3 gene transcription, and a KMnO4 footprint experiment showed that this stem and loop structure could be formed in vivo. We also observed dimethyl sulfate hypersensitive sites in the untranslated region around nucleotide +50 in MCF-7 but not in KB cells. These findings indicate that Gal NAc-T3 gene expression is regulated by multiple systems, including transcription factor binding sites and a stem-and-loop structure, and that this regulation is restricted to cell lines derived from epithelial gland adenocarcinomas but not cells derived from nonsecretory epithelial tissue carcinomas. In addition, our immunohistochemical results suggest that our anti-Gal NAc-T3 antibody may be useful for diagnostic purposes in the early stages of breast cancer.

摘要

UDP-N-乙酰-α-D-半乳糖胺:多肽N-乙酰半乳糖胺基转移酶-3(Gal NAc-T3)基因是Gal NAc转移酶基因家族的成员之一,以组织特异性方式表达。为阐明该基因的功能,我们聚焦于基因表达调控的分子机制。我们克隆了Gal NAc-T3 cDNA,并利用其证明Gal NAc-T3 mRNA在源自分泌性上皮组织腺癌的肿瘤细胞系中表达,而在源自膀胱和表皮样癌的细胞系中不表达。使用针对Gal NAc-T3的多克隆抗体,我们观察到腺癌而非非腺癌细胞系以及乳腺癌细胞而非正常乳腺组织中有蛋白表达。我们利用Gal NAc-T3 cDNA分离出三个重叠的基因组克隆,其包含人Gal NAc-T3基因的5'部分,并对第一个外显子周围1.6 kb进行了测序。使用荧光素酶基因的瞬时表达分析表明,MCF-7细胞中的启动子活性远高于KB细胞。体内足迹实验显示MCF-7细胞中一个远端GC盒、一个NRF-1位点和一个AP-2位点受到显著保护。一个从核苷酸-103延伸至核苷酸-165并与这些转录因子结合位点相邻的新型茎环结构似乎在调节Gal NAc-T3基因转录中发挥作用,高锰酸钾足迹实验表明该茎环结构可在体内形成。我们还在MCF-7细胞而非KB细胞中核苷酸+50周围的非翻译区观察到硫酸二甲酯超敏位点。这些发现表明Gal NAc-T3基因表达受多种系统调控,包括转录因子结合位点和茎环结构,且这种调控仅限于源自上皮腺腺癌的细胞系,而非源自非分泌性上皮组织癌的细胞。此外,我们的免疫组织化学结果表明,我们的抗Gal NAc-T3抗体可能有助于乳腺癌早期诊断。

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