首页> 外文期刊>Nucleic Acids Research >An in vitro screening technique for DNA polymerases that can incorporate modified nucleotides. Pseudo-thymidine as a substrate for thermostable polymerases.
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An in vitro screening technique for DNA polymerases that can incorporate modified nucleotides. Pseudo-thymidine as a substrate for thermostable polymerases.

机译:可以整合修饰核苷酸的DNA聚合酶的体外筛选技术。伪胸苷为热稳定聚合酶的底物。

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摘要

DNA polymerases are desired that incorporate modified nucleotides into DNA with diminished pausing, premature termination and infidelity. Reported here is a simple in vitro assay to screen for DNA polymerases that accept modified nucleotides based on a set of primer extension reactions. In combination with the scintillation proximity assay (SPA[trade]), this allows rapid and simple screening of enzymes for their ability to elongate oligonucleotides in the presence of unnatural nucleotides. A proof of the concept is obtained using pseudo-thymidine (psiT), the C-nucleoside analog of thymidine, as the unnatural substrate. The conformational properties of psiT arising from the carbon-carbon bond between the sugar and the base make it an interesting probe for the importance of conformational restraints in the active site of polymerases during primer elongation. From a pool of commercially available thermostable polymerases, the assay identified Taq DNA polymerase as the most suitable enzyme for the PCR amplification of oligonucleotides containing psiT. Subsequent experiments analyzing PCR performance and fidelity of Taq DNA polymerase acting on psiT are presented. This is the first time that PCR has been performed with a C-nucleoside.
机译:需要DNA聚合酶,其将修饰的核苷酸掺入DNA,同时具有减少的停顿,过早终止和不忠。此处报道的是一种简单的体外测定方法,用于基于一组引物延伸反应来筛选可接受修饰核苷酸的DNA聚合酶。与闪烁邻近测定法(SPA [trade])结合使用,可以在存在非天然核苷酸的情况下快速简便地筛选酶延长寡核苷酸的能力。使用伪胸苷(psiT)(胸苷的C核苷类似物)作为非天然底物可获得该概念的证明。由糖和碱之间的碳-碳键产生的psi​​T的构象性质使其成为引物延伸过程中聚合酶活性位点构象限制重要性的有趣探针。从一组可商购的热稳定聚合酶中,该分析鉴定出Taq DNA聚合酶是最适合PCR扩增包含psiT的寡核苷酸的酶。提出了后续实验,分析了PCR性能和作用于psiT的Taq DNA聚合酶的保真度。这是第一次使用C-核苷进行PCR。

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