Genomic Structure of Mouse Copper Chaperone, 00×17

Yoshinori Takahashi, K. Kako, K. Ohmura, K. Tsumori, Y. Ohmasa, Shin-ichi Kashiwabara, T. Baba, Eisuke Munekatat
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引用次数: 4

Abstract

Cox17p was first cloned as a cytoplasmic copper chaperone from yeast mutant and recent works suggested the existence of mammalian homologues. Previous report has shown that a gel filtration fraction of heart extract containing porcine Coxl7p peptide promoted the survival of NIH3T3 fibroblast cells. In the present study, we first cloned DNA fragments of the mouse COX17 gene. The mouse COX17 spans ∼6kb and consists of three exons. It was mapped to the center of chromosome 16, using a radiation hybrid-mapping panel. The major transcription start site is 80 bp upstream of the ATG initiation codon as determined by rapid amplification of cDNA ends (5′-RACE) analysis. Two potential polyadenylation sites are 3233 and 3293 bp downstream of the termination codon, respectively. Transient transfection of reporter plasmids containing portions of the mouse COX17 5′-flanking region into AtT-20 and NIH3T3 cells allowed the localization of the essential promoter to a 0.8 kb region upstream of the transcription starting site. Furthermore, the transfected luciferase activity was much higher in AtT-20 than NIH3T3. According to sequence analysis of the –0.8 kb 5′-flanking region, GC rich segments including consensus sequences for binding of the transcription factor Sp1, but no The TATAICAAT boxes, exist in the region of the transcription start site. Besides the GC box, binding sites for NRF-1 and 2 known as specific transcription factors for COX subunits are also localized around the transcription starting site.
小鼠铜伴侣蛋白的基因组结构,00×17
Cox17p最初是作为细胞质铜伴侣蛋白从酵母突变体中克隆出来的,最近的研究表明它在哺乳动物中也存在同源物。先前的报道表明,含有猪Coxl7p肽的心脏提取物的凝胶过滤部分促进了NIH3T3成纤维细胞的存活。在本研究中,我们首先克隆了小鼠COX17基因的DNA片段。小鼠COX17全长约6kb,由三个外显子组成。它被定位到16号染色体的中心,使用辐射混合制图面板。通过cDNA末端快速扩增(5 ' -RACE)分析,主要转录起始位点位于ATG起始密码子上游80 bp处。两个潜在的聚腺苷化位点分别位于终止密码子下游3233和3293 bp处。将含有小鼠COX17 5’侧区部分的报告质粒瞬时转染到at -20和NIH3T3细胞中,可以将基本启动子定位在转录起始位点上游0.8 kb的区域。转染后的at -20荧光素酶活性明显高于NIH3T3。根据-0.8 kb 5’侧区序列分析,在转录起始位点区域存在富含GC的片段,包括转录因子Sp1结合的一致序列,但不存在TATAICAAT盒。除了GC盒外,NRF-1和nrf - 2的结合位点(COX亚基特异性转录因子)也位于转录起始位点附近。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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