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本文引用的文献

1
The mutational specificity of two Escherichia coli dnaE antimutator alleles as determined from lacI mutation spectra.通过乳糖抑制蛋白(lacI)突变谱确定的两个大肠杆菌dnaE抗突变等位基因的突变特异性。
Genetics. 1993 Aug;134(4):1031-8. doi: 10.1093/genetics/134.4.1031.
2
Mutants of Escherichia coli with increased fidelity of DNA replication.DNA复制保真度提高的大肠杆菌突变体。
Genetics. 1993 Aug;134(4):1023-30. doi: 10.1093/genetics/134.4.1023.
3
A separate editing exonuclease for DNA replication: the epsilon subunit of Escherichia coli DNA polymerase III holoenzyme.用于DNA复制的一种独立编辑外切核酸酶:大肠杆菌DNA聚合酶III全酶的ε亚基。
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Cloning and identification of the product of the dnaE gene of Escherichia coli.大肠杆菌dnaE基因产物的克隆与鉴定
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Bacteriophage PRD1 DNA polymerase: evolution of DNA polymerases.噬菌体PRD1 DNA聚合酶:DNA聚合酶的进化
Proc Natl Acad Sci U S A. 1987 Dec;84(23):8287-91. doi: 10.1073/pnas.84.23.8287.
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DNA replication fidelity: kinetics and thermodynamics.DNA复制保真度:动力学与热力学
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High-copy-number and low-copy-number plasmid vectors for lacZ alpha-complementation and chloramphenicol- or kanamycin-resistance selection.用于lacZα互补以及氯霉素或卡那霉素抗性筛选的高拷贝数和低拷贝数质粒载体。
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Sequence analysis of the Escherichia coli dnaE gene.大肠杆菌dnaE基因的序列分析。
J Bacteriol. 1987 Dec;169(12):5735-44. doi: 10.1128/jb.169.12.5735-5744.1987.
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Using mini-prep plasmid DNA for sequencing double stranded templates with Sequenase.使用小量制备的质粒DNA,以Sequenase对双链模板进行测序。
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Kinetic mechanism whereby DNA polymerase I (Klenow) replicates DNA with high fidelity.DNA聚合酶I(克列诺片段)以高保真度复制DNA的动力学机制。
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大肠杆菌DNA聚合酶IIIα亚基中的抗突变突变:确定相关突变并与其他DNA聚合酶进行比对

Antimutator mutations in the alpha subunit of Escherichia coli DNA polymerase III: identification of the responsible mutations and alignment with other DNA polymerases.

作者信息

Fijalkowska I J, Schaaper R M

机构信息

Laboratory of Molecular Genetics, National Institute of Environmental Health Sciences, Research Triangle Park, North Carolina 27709.

出版信息

Genetics. 1993 Aug;134(4):1039-44. doi: 10.1093/genetics/134.4.1039.

DOI:10.1093/genetics/134.4.1039
PMID:8375647
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1205572/
Abstract

The dnaE gene of Escherichia coli encodes the DNA polymerase (alpha subunit) of the main replicative enzyme, DNA polymerase III holoenzyme. We have previously identified this gene as the site of a series of seven antimutator mutations that specifically decrease the level of DNA replication errors. Here we report the nucleotide sequence changes in each of the different antimutator dnaE alleles. For each a single, but different, amino acid substitution was found among the 1,160 amino acids of the protein. The observed substitutions are generally nonconservative. All affected residues are located in the central one-third of the protein. Some insight into the function of the regions of polymerase III containing the affected residues was obtained by amino acid alignment with other DNA polymerases. We followed the principles developed in 1990 by M. Delarue et al. who have identified in DNA polymerases from a large number of prokaryotic and eukaryotic sources three highly conserved sequence motifs, which are suggested to contain components of the polymerase active site. We succeeded in finding these three conserved motifs in polymerase III as well. However, none of the amino acid substitutions responsible for the antimutator phenotype occurred at these sites. This and other observations suggest that the effect of these mutations may be exerted indirectly through effects on polymerase conformation and/or DNA/polymerase interactions.

摘要

大肠杆菌的dnaE基因编码主要复制酶DNA聚合酶III全酶的DNA聚合酶(α亚基)。我们之前已将该基因鉴定为一系列七个抗突变基因的位点,这些基因特异性地降低了DNA复制错误的水平。在此我们报告每个不同抗突变dnaE等位基因中的核苷酸序列变化。在该蛋白质的1160个氨基酸中,每个都发现了一个单一但不同的氨基酸替换。观察到的替换通常是非保守的。所有受影响的残基都位于蛋白质的中央三分之一区域。通过与其他DNA聚合酶进行氨基酸比对,对包含受影响残基的聚合酶III区域的功能有了一些了解。我们遵循了M. Delarue等人在1990年提出的原则,他们在大量原核和真核来源的DNA聚合酶中鉴定出三个高度保守的序列基序,这些基序被认为包含聚合酶活性位点的组成部分。我们也成功地在聚合酶III中找到了这三个保守基序。然而,导致抗突变表型的氨基酸替换均未发生在这些位点。这一观察结果及其他观察结果表明,这些突变的影响可能是通过对聚合酶构象和/或DNA/聚合酶相互作用的影响而间接发挥作用的。