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Enhanced multiplex genome engineering through co-operative oligonucleotide co-selection

机译:通过合作寡核苷酸共选来增强多重基因组工程

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Genome-scale engineering of living organisms requires precise and economical methods to efficiently modify many loci within chromosomes. One such example is the directed integration of chemically synthesized single-stranded deoxyribonucleic acid (oligonucleotides) into the chromosome of Escherichia coli during replication. Herein, we present a general co-selection strategy in multiplex genome engineering that yields highly modified cells. We demonstrate that disparate sites throughout the genome can be easily modified simultaneously by leveraging selectable markers within 500 kb of the target sites. We apply this technique to the modification of 80 sites in the E. coli genome.
机译:生物体的基因组规模工程需要精确而经济的方法,以有效地修饰染色体内的许多基因座。一个这样的例子是在复制过程中化学合成的单链脱氧核糖核酸(寡核苷酸)直接整合到大肠杆菌的染色体中。在本文中,我们提出了在多重基因组工程中产生高度修饰细胞的通用共选策略。我们证明通过利用靶位点500 kb内的选择标记,可以轻松地同时修饰整个基因组中的不同位点。我们将此技术应用于大肠杆菌基因组中80个位点的修饰。

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