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细菌 DNA 聚合酶参与寡核苷酸重组。

Bacterial DNA polymerases participate in oligonucleotide recombination.

机构信息

Molecular Control and Genetics Section, Gene Regulation and Chromosome Biology, Frederick National Laboratory for Cancer Research, Frederick, MD 21702, USA.

出版信息

Mol Microbiol. 2013 Jun;88(5):906-20. doi: 10.1111/mmi.12231. Epub 2013 May 2.

Abstract

Synthetic single-strand oligonucleotides (oligos) with homology to genomic DNA have proved to be highly effective for constructing designed mutations in targeted genomes, a process referred to as recombineering. The cellular functions important for this type of homologous recombination have yet to be determined. Towards this end, we have identified Escherichia coli functions that process the recombining oligo and affect bacteriophage λ Red-mediated oligo recombination. To determine the nature of oligo processing during recombination, each oligo contained multiple nucleotide changes: a single base change allowing recombinant selection, and silent changes serving as genetic markers to determine the extent of oligo processing during the recombination. Such oligos were often not incorporated into the host chromosome intact; many were partially degraded in the process of recombination. The position and number of these silent nucleotide changes within the oligo strongly affect both oligo processing and recombination frequency. Exonucleases, especially those associated with DNA Polymerases I and III, affect inheritance of the silent nucleotide changes in the oligos. We demonstrate for the first time that the major DNA polymerases (Pol I and Pol III) and DNA ligase are directly involved with oligo recombination.

摘要

合成的单链寡核苷酸(寡核苷酸)与基因组 DNA 同源,已被证明在构建靶向基因组中的设计突变方面非常有效,这一过程称为重组。但对于这种同源重组所必需的细胞功能仍有待确定。为此,我们已经确定了大肠杆菌中处理重组寡核苷酸并影响噬菌体 λ Red 介导的寡核苷酸重组的功能。为了确定重组过程中寡核苷酸的处理性质,每个寡核苷酸都包含多个核苷酸变化:一个碱基变化允许进行重组选择,而沉默变化则作为遗传标记,以确定在重组过程中寡核苷酸的处理程度。这种寡核苷酸通常不会完整地整合到宿主染色体中;许多在重组过程中被部分降解。寡核苷酸中这些沉默核苷酸变化的位置和数量强烈影响寡核苷酸的处理和重组频率。核酸外切酶,尤其是与 DNA 聚合酶 I 和 III 相关的核酸外切酶,会影响寡核苷酸中沉默核苷酸变化的遗传。我们首次证明主要的 DNA 聚合酶(Pol I 和 Pol III)和 DNA 连接酶直接参与了寡核苷酸的重组。

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