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DNA聚合酶催化将非模板额外核苷酸添加到DNA片段的3'末端。

DNA polymerase-catalyzed addition of nontemplated extra nucleotides to the 3' end of a DNA fragment.

作者信息

Hu G

机构信息

Massachusetts Institute of Technology, Whitaker College of Health Sciences and Technology, Cambridge 02139.

出版信息

DNA Cell Biol. 1993 Oct;12(8):763-70. doi: 10.1089/dna.1993.12.763.

Abstract

Some prokaryotic and eukaryotic DNA polymerases are capable of adding an additional nontemplated nucleotide residue at the 3' end of a DNA fragment (Clark et al., 1987; Clark, 1988). The extra nucleotide at the 3' end of the PCR product has been shown to be a critical factor determining the efficiency of cloning PCR products into plasmids and can affect mutation analyses with a PCR-denaturing gradient gel electrophoresis (DGGE) approach (Pfeiffer and Hu, 1993). In the present work, the ability of various DNA polymerases to add an extra nontemplated nucleotide at the 3' end of DNA was studied. The results show that out of the eight studied enzymes, five can add, with varying efficiencies, an extra nucleotide residue at the 3' end of DNA. Which extra nucleotide is added depends on the terminal residue and the DNA polymerase. Among the enzymes, thermostable Pfu DNA polymerase is found to be the best choice for PCR due to its relatively high fidelity (Scott et al., 1991; Coller, unpublished), and ability to produce blunt-ended DNA fragments. The relationship between the DNA polymerases' ability to add an extra nucleotide and their 3'-->5' exonuclease activity is also discussed.

摘要

一些原核生物和真核生物的DNA聚合酶能够在DNA片段的3'端添加一个额外的非模板核苷酸残基(Clark等人,1987年;Clark,1988年)。PCR产物3'端的额外核苷酸已被证明是决定将PCR产物克隆到质粒中的效率的关键因素,并且会影响采用PCR-变性梯度凝胶电泳(DGGE)方法进行的突变分析(Pfeiffer和Hu,1993年)。在本研究中,研究了各种DNA聚合酶在DNA的3'端添加额外非模板核苷酸的能力。结果表明,在所研究的8种酶中,有5种能够以不同的效率在DNA的3'端添加一个额外的核苷酸残基。添加的是哪种额外核苷酸取决于末端残基和DNA聚合酶。在这些酶中,由于其相对较高的保真度(Scott等人,1991年;Coller,未发表)以及产生平端DNA片段的能力,耐热的Pfu DNA聚合酶被发现是PCR的最佳选择。还讨论了DNA聚合酶添加额外核苷酸的能力与其3'→5'核酸外切酶活性之间的关系。

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