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首页> 外文期刊>Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems >A step forward: Compatible and dual-inducible expression vectors for gene co-expression in Corynebacterium glutamicum
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A step forward: Compatible and dual-inducible expression vectors for gene co-expression in Corynebacterium glutamicum

机译:前进:用于谷氨酸杆菌基因共同表达的兼容和双诱导的表达载体

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摘要

The Gram-positive bacterium Corynebacterium glutamicum represents a promising platform for the production of amino acids, organic acids, and other bio-products. However, the availability of only few expression vectors limits its use for production purposes, using metabolic engineering approaches when co-expression of several target genes is desired. To widen the scope for co-expression, the pCG1/p15A and pBL1/colEl replicons were employed to construct the two differentially-inducible and compatible expression vectors pRG_Duet1 and pRG_Duet2. To functionally validate these newly constructed expression vectors, target genes for easily measurable enzymes were cloned and over-expression of these genes was investigated using respective enzyme assays. Furthermore, functionality and co-existence of the pCG1-based C. glutamicum - E. coli shuttle vector pRG_Duet1 were confirmed with pBL1-based expression vectors pRG_Duet2 and pEKEx2, using co-transformation and enzyme assays. The novel shuttle expression vectors pRGDuet1 and pRG_Duet2 are attractive additions to the existing set of vectors for co-expression studies and metabolic engineering of C. glutamicum.
机译:革兰氏阳性细菌棒状杆菌谷氨酸代表了用于生产氨基酸,有机酸和其他生物产物的有希望的平台。然而,只有少量表达向量的可用性限制了其用于生产目的的用途,当需要代谢工程方法时,当需要进行几种靶基因的共同表达时。为了扩大共表达的范围,采用PCG1 / P15A和PBL1 / COLEL复制子来构建两个差异诱导和兼容的表达载体PRG_DUET1和PRG_DUET2。为了在功能上验证这些新构建的表达载体,克隆易可测量酶的靶基因并使用各种酶测定研究这些基因的过表达。此外,使用共转化和酶测定,用PBL1基表达载体PRG_DUET2和PEKEx2确认PCG1的C.谷氨酰胺-E.Coli梭载体PRG_Duet1的功能和共存。新型梭式表达载体PRGDUET1和PRG_DUET2是对现有的C.谷氨酰胺的共表达研究和代谢工程的现有载体的吸引力。

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