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在产黄青霉中,编码酵母氨酸还原酶的lys7基因失活,导致次生代谢物前体哌啶-6-羧酸和哌可酸从α-氨基己二酸积累。

Inactivation of the lys7 gene, encoding saccharopine reductase in Penicillium chrysogenum, leads to accumulation of the secondary metabolite precursors piperideine-6-carboxylic acid and pipecolic acid from alpha-aminoadipic acid.

作者信息

Naranjo Leopoldo, Martín de Valmaseda Eva, Casqueiro Javier, Ullán Ricardo V, Lamas-Maceiras Mónica, Bañuelos Oscar, Martín Juan F

机构信息

Area de Microbiología, Facultad de Ciencias Biológicas y Ambientales, Universidad de León, 24071 León, Spain.

出版信息

Appl Environ Microbiol. 2004 Feb;70(2):1031-9. doi: 10.1128/AEM.70.2.1031-1039.2004.

Abstract

Pipecolic acid serves as a precursor of the biosynthesis of the alkaloids slaframine and swainsonine (an antitumor agent) in some fungi. It is not known whether other fungi are able to synthesize pipecolic acid. Penicillium chrysogenum has a very active alpha-aminoadipic acid pathway that is used for the synthesis of this precursor of penicillin. The lys7 gene, encoding saccharopine reductase in P. chrysogenum, was target inactivated by the double-recombination method. Analysis of a disrupted strain (named P. chrysogenum SR1-) showed the presence of a mutant lys7 gene lacking about 1,000 bp in the 3'-end region. P. chrysogenum SR1- lacked saccharopine reductase activity, which was recovered after transformation of this mutant with the intact lys7 gene in an autonomously replicating plasmid. P. chrysogenum SR1- was a lysine auxotroph and accumulated piperideine-6-carboxylic acid. When mutant P. chrysogenum SR1- was grown with L-lysine as the sole nitrogen source and supplemented with DL-alpha-aminoadipic acid, a high level of pipecolic acid accumulated intracellularly. A comparison of strain SR1- with a lys2-defective mutant provided evidence showing that P. chrysogenum synthesizes pipecolic acid from alpha-aminoadipic acid and not from L-lysine catabolism.

摘要

在一些真菌中,哌啶酸是生物碱疯草毒素和苦马豆素(一种抗肿瘤剂)生物合成的前体。尚不清楚其他真菌是否能够合成哌啶酸。产黄青霉具有非常活跃的α-氨基己二酸途径,该途径用于合成青霉素的这种前体。产黄青霉中编码酵母氨酸还原酶的lys7基因通过双重组方法进行靶向失活。对一个破坏菌株(命名为产黄青霉SR1-)的分析表明,存在一个在3'-末端区域缺失约1000 bp的突变型lys7基因。产黄青霉SR1-缺乏酵母氨酸还原酶活性,在用自主复制质粒中的完整lys7基因转化该突变体后,该活性得以恢复。产黄青霉SR1-是赖氨酸营养缺陷型,积累了哌啶-6-羧酸。当突变型产黄青霉SR1-以L-赖氨酸作为唯一氮源生长并补充DL-α-氨基己二酸时,细胞内积累了高水平的哌啶酸。将SR1-菌株与lys2缺陷型突变体进行比较,提供了证据表明产黄青霉从α-氨基己二酸而不是从L-赖氨酸分解代谢合成哌啶酸。

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