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用携带大鼠细胞色素P-450MC cDNA的表达质粒转化的酿酒酵母细胞的单加氧酶活性。

Monooxygenase activity of Saccharomyces cerevisiae cells transformed with expression plasmids carrying rat cytochrome P-450MC cDNA.

作者信息

Sakaki T, Oeda K, Yabusaki Y, Ohkawa H

出版信息

J Biochem. 1986 Mar;99(3):741-9. doi: 10.1093/oxfordjournals.jbchem.a135533.

Abstract

The recombinant plasmids pAMC1 and pJMC1 were constructed; the former contained the cytochrome P-450MC (P-450MC) cDNA expression unit consisting of yeast alcohol dehydrogenase I (ADH) promoter, rat P-450MC cDNA and ADH terminator, and the Leu 2 marker gene, and the latter contained the same expression unit and the leu 2-d gene. Saccharomyces cerevisiae AH22 cells transformed with each of the recombinant plasmids were examined for plasmid copy number, P-450MC mRNA level, P-450MC content, and monooxygenase activity. The S. cerevisiae AH22/pJMC1 cells contained about 2-fold higher levels of the plasmid, P-450MC mRNA, and P-450MC than the AH22/pAMC1 cells. Monooxygenase activity towards 7-ethoxycoumarin and acetanilide of the AH22/pJMC1 cells was 1.7-fold and 1.5-fold higher than that of the AH22/pAMC1 cells, respectively, whereas the activity of the AH22/pAMC1 cells towards 7-ethoxycoumarin and acetanilide was more than 1,000-fold 10-fold higher than that of the control AH22/pAAH5 cells which contain no P-450MC cDNA, respectively. Therefore, it is likely that monooxygenase activity of the AH22 cells carrying rat P-450MC cDNA was approximately proportional to the expression level of P-450MC cDNA.

摘要

构建了重组质粒pAMC1和pJMC1;前者包含由酵母乙醇脱氢酶I(ADH)启动子、大鼠P-450MC cDNA和ADH终止子组成的细胞色素P-450MC(P-450MC)cDNA表达单元,以及亮氨酸2标记基因,后者包含相同的表达单元和亮氨酸2-d基因。对用每种重组质粒转化的酿酒酵母AH22细胞进行了质粒拷贝数、P-450MC mRNA水平、P-450MC含量和单加氧酶活性的检测。酿酒酵母AH22/pJMC1细胞所含的质粒、P-450MC mRNA和P-450MC水平比AH22/pAMC1细胞高约2倍。AH22/pJMC1细胞对7-乙氧基香豆素和乙酰苯胺的单加氧酶活性分别比AH22/pAMC1细胞高1.7倍和1.5倍,而AH22/pAMC1细胞对7-乙氧基香豆素和乙酰苯胺的活性分别比不含P-450MC cDNA的对照AH22/pAAH5细胞高1000多倍和10倍。因此,携带大鼠P-450MC cDNA的AH22细胞的单加氧酶活性可能与P-450MC cDNA的表达水平大致成正比。

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