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通过基于DNA微阵列的新型靶基因鉴定提高谷氨酸棒杆菌的赖氨酸产量。

Improving lysine production by Corynebacterium glutamicum through DNA microarray-based identification of novel target genes.

作者信息

Sindelar Georg, Wendisch Volker F

机构信息

Institute of Biotechnology I, Research Center Jülich, Julich, Germany.

出版信息

Appl Microbiol Biotechnol. 2007 Sep;76(3):677-89. doi: 10.1007/s00253-007-0916-x. Epub 2007 Mar 16.

DOI:10.1007/s00253-007-0916-x
PMID:17364200
Abstract

For the biotechnological production of L: -lysine, mainly strains of Corynebacterium glutamicum are used, which have been obtained by classical mutagenesis and screening or selection or by metabolic engineering. Gene targets for the amplification and deregulation of the lysine biosynthesis pathway, for the improvement of carbon precursor supply and of nicotinamide adenine dinucleotide phosphate (reduced form) (NADPH) regeneration, are known. To identify novel target genes to improve lysine production, the transcriptomes of the classically obtained lysine producing strain MH20-22B and several other C. glutamicum strains were compared. As lysine production by the classically obtained strain, which possesses feedback-resistant aspartokinase and is leucine auxotrophic, exceeds that of a genetically defined leucine auxotrophic wild-type derivative possessing feedback-resistant aspartokinase, additional traits beneficial for lysine production are present. NCgl0855, putatively encoding a methyltransferase, and the amtA-ocd-soxA operon, encoding an ammonium uptake system, a putative ornithine cyclodeaminase and an uncharacterized enzyme, were among the genes showing increased expression in the classically obtained strain irrespective of the presence of feedback-resistant aspartokinase. Lysine production could be improved by about 40% through overexpression of NCgl0855 or the amtA-ocd-soxA operon. Thus, novel target genes for the improvement of lysine production could be identified in a discovery-driven approach based on global gene expression analysis.

摘要

对于L-赖氨酸的生物技术生产,主要使用谷氨酸棒杆菌菌株,这些菌株是通过经典诱变、筛选或选择或代谢工程获得的。赖氨酸生物合成途径的扩增和去调控、碳前体供应的改善以及烟酰胺腺嘌呤二核苷酸磷酸(还原型)(NADPH)再生的基因靶点是已知的。为了鉴定提高赖氨酸产量的新靶点基因,比较了经典获得的赖氨酸生产菌株MH20-22B和其他几种谷氨酸棒杆菌菌株的转录组。由于经典获得的具有抗反馈天冬氨酸激酶且为亮氨酸营养缺陷型的菌株的赖氨酸产量超过了具有抗反馈天冬氨酸激酶的遗传定义的亮氨酸营养缺陷型野生型衍生物,所以存在其他有利于赖氨酸生产的性状。假定编码甲基转移酶的NCgl0855以及编码铵摄取系统、假定的鸟氨酸环脱氨酶和一种未鉴定酶的amtA-ocd-soxA操纵子,是在经典获得的菌株中无论是否存在抗反馈天冬氨酸激酶都表现出表达增加的基因。通过过表达NCgl0855或amtA-ocd-soxA操纵子,赖氨酸产量可提高约40%。因此,基于全局基因表达分析的发现驱动方法可鉴定出提高赖氨酸产量的新靶点基因。

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