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人类细胞色素P - 450c基因的结构与药物诱导性

Structure and drug inducibility of the human cytochrome P-450c gene.

作者信息

Kawajiri K, Watanabe J, Gotoh O, Tagashira Y, Sogawa K, Fujii-Kuriyama Y

出版信息

Eur J Biochem. 1986 Sep 1;159(2):219-25. doi: 10.1111/j.1432-1033.1986.tb09857.x.

Abstract

A human genomic clone (lambda hP-450mc-1), highly homologous to the rat cytochrome P-450c gene, was isolated and analyzed for the complete nucleotide sequence. The gene structure coincides with that of a recently reported human gene isolated from genomic DNA of a human breast carcinoma cell line, MCF-7 [Jaiswal, A.K., Gonzalez, F.J. & Nebert, D.W. (1985) Nucleic Acids Res. 13, 4503-4520] with notable exceptions in the first intron: a 320-base-pair fragment is inserted and a 650-base-pair fragment is deleted in the gene examined in the present study. The 320-base-pair insert appears to contain a moderately repetitive sequence (approx. 140 copies) in the human genome. The 650-base-pair fragment, present in intron 1 of the reported sequence, is dislocated in the lambda hP-450mc-1 to about 10(4) base pairs upstream from the putative transcription initiation site. The results of Southern blot analysis using human total DNA were compatible with the gene structure of lambda hP-450mc-1. A fusion gene, which was constructed by ligating the 5' flanking region of the gene to the structural gene for prokaryotic chloramphenicol acetyltransferase (CAT), inducibly expressed the CAT activity in mouse Hepa-1 cells in response to administered methylcholanthrene, indicating that the isolated human gene is indeed of methylcholanthrene inducibility.

摘要

分离出一个与大鼠细胞色素P-450c基因高度同源的人类基因组克隆(λhP - 450mc - 1),并对其完整核苷酸序列进行了分析。该基因结构与最近从人乳腺癌细胞系MCF - 7的基因组DNA中分离出的人类基因结构一致[贾斯瓦尔,A.K.,冈萨雷斯,F.J. & 内伯特,D.W.(1985年)《核酸研究》13卷,4503 - 4520页],但在第一个内含子中有显著差异:在本研究检测的基因中插入了一个320个碱基对的片段,缺失了一个650个碱基对的片段。320个碱基对的插入片段似乎包含人类基因组中的一个中度重复序列(约140个拷贝)。报道序列的内含子1中存在的650个碱基对片段,在λhP - 450mc - 1中移位到推定转录起始位点上游约10⁴个碱基对处。用人总DNA进行的Southern印迹分析结果与λhP - 450mc - 1的基因结构相符。通过将该基因的5'侧翼区与原核氯霉素乙酰转移酶(CAT)的结构基因连接构建的融合基因,在给予甲基胆蒽后可诱导小鼠Hepa - 1细胞中CAT活性表达,表明分离出的人类基因确实具有甲基胆蒽诱导性。

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