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白亚麻两种不同细胞悬浮培养物中的芳基四氢萘木脂素形成:脱氧鬼臼毒素6-羟化酶,一种6-甲氧基鬼臼毒素形成的关键酶。

Aryltetralin-lignan formation in two different cell suspension cultures of Linum album: deoxypodophyllotoxin 6-hydroxylase, a key enzyme for the formation of 6-methoxypodophyllotoxin.

作者信息

Federolf Katja, Alfermann A Wilhelm, Fuss Elisabeth

机构信息

Institut für Entwicklungs- und Molekularbiologie der Pflanzen, Heinrich-Heine-Universität Düsseldorf, Universitätsstr. 1, 40225 Düsseldorf, Germany.

出版信息

Phytochemistry. 2007 May;68(10):1397-406. doi: 10.1016/j.phytochem.2007.02.031. Epub 2007 Apr 20.

Abstract

Suspension cultures initiated from two different Linum album seedlings accumulate either podophyllotoxin (PTOX, 2.6 mg/g DW) or 6-methoxypodophyllotoxin (6MPTOX, 5.4 mg/g DW) as main lignans. Two molecules of coniferyl alcohol are dimerized to pinoresinol which is converted via several steps into deoxypodophyllotoxin (DOP) which seems to be the branching point to PTOX or 6MPTOX biosynthesis. DOP is hydroxylated at position 7 to give PTOX by deoxypodophyllotoxin 7-hydroxylase (DOP7H). In contrast, 6MPTOX biosynthesis is achieved by DOP hydroxylation at position 6 to beta-peltatin by the cytochrome P450 enzyme deoxypodophyllotoxin 6-hydroxylase (DOP6H). The following methylation to beta-peltatin-A-methylether is catalyzed by beta-peltatin 6-O-methyltransferase (betaP6OMT) from which 6MPTOX is formed by hydroxylation at position 7 by beta-peltatin-A-methylether 7-hydroxylase (PAM7H). DOP6H and betaP6OMT could be characterized in protein extracts from cell cultures of L. flavum and L. nodiflorum, respectively, and here in L. album for the first time. DOP7H and PAM7H activities could not yet be detected with protein extracts. Experiments of feeding DOP together with inhibitors of cytochrome P450 depending as well as dioxygenase enzymes were performed in order to shed light on the type of DOP7H and PAM7H. Growth parameters and specific activities of enzymes from the phenylpropane as well as the lignan specific biosynthetic pathway were measured during a culture period of 16 days. From the enzymes studied only the DOP6H showed a differential activity sustaining the hypothesis that this enzyme is responsible for the differential lignan accumulation in both cell lines.

摘要

由两种不同的亚麻幼苗起始的悬浮培养物分别积累鬼臼毒素(PTOX,2.6毫克/克干重)或6-甲氧基鬼臼毒素(6MPTOX,5.4毫克/克干重)作为主要木脂素。两分子松柏醇二聚形成松脂醇,松脂醇经几步转化为脱氧鬼臼毒素(DOP),DOP似乎是PTOX或6MPTOX生物合成的分支点。DOP在7位被脱氧鬼臼毒素7-羟化酶(DOP7H)羟基化生成PTOX。相反,6MPTOX的生物合成是通过细胞色素P450酶脱氧鬼臼毒素6-羟化酶(DOP6H)将DOP在6位羟基化生成β-盾叶鬼臼毒素来实现的。随后的甲基化生成β-盾叶鬼臼毒素-A-甲基醚由β-盾叶鬼臼毒素6-O-甲基转移酶(βP6OMT)催化,β-盾叶鬼臼毒素-A-甲基醚7-羟化酶(PAM7H)在7位羟基化生成6MPTOX。DOP6H和βP6OMT分别可以在淡黄亚麻和无梗亚麻细胞培养物的蛋白质提取物中得到表征,这里首次在亚麻中得到表征。蛋白质提取物尚未检测到DOP7H和PAM7H活性。进行了将DOP与细胞色素P450依赖性抑制剂以及双加氧酶一起投喂的实验,以阐明DOP7H和PAM7H的类型。在16天的培养期内测量了来自苯丙烷以及木脂素特异性生物合成途径的酶的生长参数和比活性。在所研究的酶中,只有DOP6H表现出差异活性,支持了该酶负责两种细胞系中木脂素差异积累的假说。

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