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烟草中N-甲基腐胺氧化酶的分子克隆

Molecular cloning of N-methylputrescine oxidase from tobacco.

作者信息

Katoh Akira, Shoji Tsubasa, Hashimoto Takashi

机构信息

Nara Institute of Science and Technology, Graduate School of Biological Sciences, 8916-5 Takayama, Ikoma, Nara, 630-0192, Japan.

出版信息

Plant Cell Physiol. 2007 Mar;48(3):550-4. doi: 10.1093/pcp/pcm018. Epub 2007 Feb 5.

Abstract

Nicotine biosynthesis in Nicotiana species requires an oxidative deamination of N-methylputrescine, catalyzed by N-methylputrescine oxidase (MPO). In a screen for tobacco genes that were down-regulated in a tobacco mutant with altered regulation of nicotine biosynthesis, we identified two homologous MPO cDNAs which encode diamine oxidases of a particular subclass. Tobacco MPO genes were expressed specifically in the root, and up-regulated by jasmonate treatment. Recombinant MPO protein expressed in Escherichia coli formed a homodimer and deaminated N-methylputrescine more efficiently than symmetrical diamines. These results indicate that MPO evolved from general diamine oxidases to function effectively in nicotine biosynthesis.

摘要

烟草属植物中的尼古丁生物合成需要由N-甲基腐胺氧化酶(MPO)催化的N-甲基腐胺的氧化脱氨反应。在对尼古丁生物合成调控改变的烟草突变体中下调的烟草基因进行筛选时,我们鉴定出两个同源的MPO cDNA,它们编码特定亚类的二胺氧化酶。烟草MPO基因在根中特异性表达,并通过茉莉酸处理上调。在大肠杆菌中表达的重组MPO蛋白形成同型二聚体,并且比对称二胺更有效地使N-甲基腐胺脱氨。这些结果表明,MPO从一般的二胺氧化酶进化而来,在尼古丁生物合成中发挥有效作用。

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