首页> 美国卫生研究院文献>Journal of Bacteriology >Amplification of bacterial genomic DNA by the polymerase chain reaction and direct sequencing after asymmetric amplification: application to the study of periplasmic permeases.
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Amplification of bacterial genomic DNA by the polymerase chain reaction and direct sequencing after asymmetric amplification: application to the study of periplasmic permeases.

机译:通过聚合酶链反应扩增细菌基因组DNA并在不对称扩增后直接测序:在周质渗透酶研究中的应用。

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摘要

The polymerase chain reaction (PCR) has been used to amplify DNA fragments by using eucaryotic genomic DNA as a template. We show that bacterial genomic DNA can be used as a template for PCR amplification. We demonstrate that DNA fragments at least as large as 4,400 base pairs can be amplified with fidelity and that the amplified DNA can be used as a substrate for most operations involving DNA. We discuss problems inherent in the direct sequencing of the amplified product, one of the important exploitations of this methodology. We have solved the problems by developing an "asymmetric amplification" method in which one of the oligonucleotide primers is used in limiting amounts, thus allowing the accumulation of single-stranded copies of only one of the DNA strands. As an illustration of the use of PCR in bacteria, we have amplified, sequenced, and subcloned several DNA fragments carrying mutations in genes of the histidine permease operon. These mutations are part of a preliminary approach to studying protein-protein interactions in transport, and their nature is discussed.
机译:通过使用真核基因组DNA作为模板,聚合酶链反应(PCR)已用于扩增DNA片段。我们表明,细菌基因组DNA可以用作PCR扩增的模板。我们证明,可以保真地扩增至少4400个碱基对的DNA片段,并且扩增的DNA可以用作大多数涉及DNA的操作的底物。我们讨论了扩增产物直接测序中固有的问题,这是该方法的重要开发之一。我们已经通过开发一种“不对称扩增”方法解决了这些问题,在该方法中,寡核苷酸引物之一以有限的量使用,从而仅使一条DNA链的单链拷贝得以积累。作为在细菌中使用PCR的例证,我们已经扩增,测序和亚克隆了几个带有组氨酸通透酶操纵子基因突变的DNA片段。这些突变是研究运输中蛋白质相互作用的初步方法的一部分,并对其性质进行了讨论。

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