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Unique Substrate Spectrum and PCR Application of Nanoarchaeum equitans Family B DNA Polymerase

机译:Nanoarchaeum equitans家族B DNA聚合酶的独特底物光谱和PCR应用

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摘要

The known archaeal family B DNA polymerases are unable to participate in the PCR in the presence of uracil. Here, we report on a novel archaeal family B DNA polymerase from Nanoarchaeum equitans that can successfully utilize deaminated bases such as uracil and hypoxanthine and on its application to PCR. N. equitans family B DNA polymerase (Neq DNA polymerase) produced λ DNA fragments up to 10 kb with an approximately 2.2-fold-lower error rate (5.53 × 10−6) than Taq DNA polymerase (11.98 × 10−6). Uniquely, Neq DNA polymerase also amplified λ DNA fragments using dUTP (in place of dTTP) or dITP (partially replaced with dGTP). To increase PCR efficiency, Taq and Neq DNA polymerases were mixed in different ratios; a ratio of 10:1 efficiently facilitated long PCR (20 kb). In the presence of dUTP, the PCR efficiency of the enzyme mixture was two- to threefold higher than that of either Taq and Neq DNA polymerase alone. These results suggest that Neq DNA polymerase and Neq plus DNA polymerase (a mixture of Taq and Neq DNA polymerases) are useful in DNA amplification and PCR-based applications, particularly in clinical diagnoses using uracil-DNA glycosylase.
机译:在尿嘧啶存在下,已知的古细菌B族DNA聚合酶不能参与PCR。在这里,我们报道了一种新的古细菌家族B DNA聚合酶,它可以成功利用脱氨基碱基(如尿嘧啶和次黄嘌呤)及其在PCR中的应用。 N. equitans家族B DNA聚合酶(Neq DNA聚合酶)产生高达10 kb的λDNA片段,其错误率(5.53×10 -6 )比Taq DNA聚合酶(11.98)低约2.2倍。 ×10 −6 )。独特的是,Neq DNA聚合酶还使用dUTP(代替dTTP)或dITP(部分被​​dGTP取代)扩增了λDNA片段。为了提高PCR效率,以不同比例混合Taq和Neq DNA聚合酶。 10:1的比率可有效促进长PCR(20 kb)。在dUTP存在下,酶混合物的PCR效率比单独的Taq和Neq DNA聚合酶高出2到3倍。这些结果表明,Neq DNA聚合酶和Neq加DNA聚合酶(Taq和Neq DNA聚合酶的混合物)可用于DNA扩增和基于PCR的应用,特别是在使用尿嘧啶DNA糖基化酶的临床诊断中。

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