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首页> 外文期刊>Molecular Biotechnology >Strain Engineering by Genome Mass Transfer: Efficient Chromosomal Trait Transfer Method Utilizing Donor Genomic DNA and Recipient Recombineering Hosts
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Strain Engineering by Genome Mass Transfer: Efficient Chromosomal Trait Transfer Method Utilizing Donor Genomic DNA and Recipient Recombineering Hosts

机译:基因组传质的菌株工程:利用供体基因组DNA和收件人重组宿主的有效染色体性状转移方法。

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摘要

Strain engineering, like cloning, is a fundamental technology used to confer new traits onto existing strains. While effective methods for trait development through gene modification within strains have been developed, methods for trait transfer between Escherichia coli strains to create complex strains are needed. We report herein the development of genome mass transfer (GMT), a broadly applicable new strain engineering methodology enabling rapid trait transfer from a donor strain into a recombineering gene-expressing recipient strain. GMT utilizes electroporation of donor chromosomal DNA into a recombineering recipient cell for precise trait transfer. GMT transfer of traits between E. coli strains can be used to rapidly assemble new strains incorporating combinations of marked gene knockouts, for example, utilizing the existing E. coli K-12 Keio gene knockout collection as source target genes. Optional use of random primed isothermal amplified DNA eliminates the need for initial DNA purification, affording high throughput application. This allows unprecedented simplicity and speed for rational design engineering of complex phenotypes in industrial strains.
机译:像克隆一样,菌株工程是一种用于向现有菌株赋予新性状的基本技术。尽管已经开发了通过菌株内的基因修饰来发展性状的有效方法,但是需要用于在大肠杆菌菌株之间转移性状以产生复杂菌株的方法。我们在此报告基因组传质(GMT)的发展,这是一种广泛适用的新菌株工程学方法,能够将快速的性状从供体菌株转移到重组基因表达受体菌株中。 GMT利用供体染色体DNA的电穿孔进入重组受体细胞以进行精确的性状转移。大肠杆菌菌株之间性状的GMT转移可用于快速组装结合了标记基因敲除组合的新菌株,例如,利用现有的大肠杆菌K-12 Keio基因敲除集合作为源靶基因。可选使用随机引物等温扩增的DNA,无需进行初始DNA纯化,可提供高通量应用。这为工业菌株中复杂表型的合理设计工程提供了前所未有的简便性和速度。

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