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A novel genetic tool for metabolic optimization of Corynebacterium glutamicum: efficient and repetitive chromosomal integration of synthetic promoter-driven expression libraries

Appl Microbiol Biotechnol. 2016; 
Shen J, Chen J, Jensen PR, Solem C.
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PCR Cloning and Subcloning … A synthetic DNA fragment (Fig S1), which contained lox66, lox71, the lysA terminator, attP, attB, and multiple cloning sites (MCSs), was designed and synthesized by GenScript. This sequence was amplified using 5′-phosphorylated primers p39 and p40 … Get A Quote

摘要

Fine-tuning the expression level of multiple genes is usually pivotal for metabolic optimization. We have developed a tool for this purpose for the important industrial workhorse Corynebacterium glutamicum that allows for the introduction of synthetic promoter-driven expression libraries of arbitrary genes. We first devised a method for introducing genetic elements into the chromosome repeatedly, relying on site-specific recombinases and the vector pJS31 serving as the carrier. The pJS31 vector contains a synthetic cassette including a phage attachment site attP for integration, a bacterial attachment site attB for subsequent integration, a multiple cloning site, and two modified loxP sites to facilitate easy r... More

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