利用靶向寡核苷酸文库和功能筛选进行基因组工程。
Genome engineering using targeted oligonucleotide libraries and functional selection.
作者信息
Diner Elie J, Garza-Sánchez Fernando, Hayes Christopher S
机构信息
Biomolecular Science and Engineering Program, University of California, Santa Barbara, Santa Barbara, CA, USA.
出版信息
Methods Mol Biol. 2011;765:71-82. doi: 10.1007/978-1-61779-197-0_5.
Abstract
The λ phage Red proteins greatly enhance homologous recombination in Escherichia coli. Red-mediated recombination or "recombineering" can be used to construct targeted gene deletions as well as to introduce point mutations into the genome. Here, we describe our method for scanning mutagenesis using recombineered oligonucleotide libraries. This approach entails randomization of specific codons within a target gene, followed by functional selection to isolate mutants. Oligonucleotide library mutagenesis has generated hundreds of novel antibiotic resistance mutations in genes encoding ribosomal proteins, and should be applicable to other systems for which functional selections exist.
摘要
λ噬菌体Red蛋白极大地增强了大肠杆菌中的同源重组。Red介导的重组或“重组工程”可用于构建靶向基因缺失以及将点突变引入基因组。在此,我们描述了使用重组寡核苷酸文库进行扫描诱变的方法。该方法需要使靶基因内的特定密码子随机化,然后进行功能筛选以分离突变体。寡核苷酸文库诱变已在编码核糖体蛋白的基因中产生了数百种新的抗生素抗性突变,并且应该适用于存在功能筛选的其他系统。
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