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哺乳动物 DNA 聚合酶 β 连续掺入荧光标记核苷酸。

Consecutive incorporation of fluorophore-labeled nucleotides by mammalian DNA polymerase beta.

机构信息

Nano-Bioanalysis Team, Health Technology Research Center, National Institute of Advanced Industrial Science and Technology, Takamatsu, Kagawa 761-0395, Japan.

出版信息

Anal Biochem. 2010 Oct 15;405(2):160-7. doi: 10.1016/j.ab.2010.06.005. Epub 2010 Jun 4.

Abstract

In the present study, we investigated mammalian polymerases that consecutively incorporate various fluorophore-labeled nucleotides. We found that rat DNA polymerase beta (pol beta) consecutively incorporated fluorophore-labeled nucleotides to a greater extent than four bacterial polymerases, Sequenase Version 2.0, Vent(R) (exo-), DNA polymerase IIIalpha and the Klenow fragment, and the mammalian polymerases DNA polymerase alpha and human DNA polymerase delta, under mesophilic conditions. Furthermore, we investigated the kinetics of correct or mismatched incorporation with labeled nucleotides during synthesis by rat pol beta. The kinetic parameters K(m) and k(cat) were measured and used for evaluating: (i) the discrimination against correct pair incorporation of labeled nucleotides relative to unlabeled nucleotides; and (ii) the fidelity for all nucleotide combinations of mismatched pairs in the presence of labeled or unlabeled nucleotides. We also investigated the effect of fluorophore-labeled nucleotides on terminal deoxynucleotidyl transferase activity of rat pol beta. We have demonstrated for the first time that mammalian pol beta can consecutively incorporate various fluorophore-labeled dNTPs. These findings suggest that pol beta is useful for high-density labeling of DNA probes and single-molecule sequencing for high-speed genome analysis.

摘要

在本研究中,我们研究了连续掺入各种荧光标记核苷酸的哺乳动物聚合酶。我们发现,在中温条件下,大鼠 DNA 聚合酶β(polβ)比四种细菌聚合酶(Sequenase Version 2.0、Vent(R)(外切)、DNA 聚合酶 IIIα和 Klenow 片段)以及哺乳动物聚合酶 DNA 聚合酶α和人 DNA 聚合酶δ更连续地掺入荧光标记核苷酸。此外,我们研究了大鼠 polβ在合成过程中用标记核苷酸进行正确或错配掺入的动力学。测量了动力学参数 K(m)和 k(cat),并用于评估:(i)相对于未标记核苷酸,标记核苷酸对正确配对掺入的选择性;和(ii)在存在标记或未标记核苷酸时,错配碱基对的所有核苷酸组合的保真度。我们还研究了荧光标记核苷酸对大鼠 polβ末端脱氧核苷酸转移酶活性的影响。我们首次证明了哺乳动物 polβ可以连续掺入各种荧光标记的 dNTP。这些发现表明 polβ可用于 DNA 探针的高密度标记和单分子测序,以实现高速基因组分析。

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