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细胞脱氧核苷三磷酸的定量。

Quantitation of cellular deoxynucleoside triphosphates.

机构信息

Department of Biology, University of Padova, 35131 Padova, Italy.

出版信息

Nucleic Acids Res. 2010 Apr;38(6):e85. doi: 10.1093/nar/gkp1141. Epub 2009 Dec 11.

Abstract

Eukaryotic cells contain a delicate balance of minute amounts of the four deoxyribonucleoside triphosphates (dNTPs), sufficient only for a few minutes of DNA replication. Both a deficiency and a surplus of a single dNTP may result in increased mutation rates, faulty DNA repair or mitochondrial DNA depletion. dNTPs are usually quantified by an enzymatic assay in which incorporation of radioactive dATP (or radioactive dTTP in the assay for dATP) into specific synthetic oligonucleotides by a DNA polymerase is proportional to the concentration of the unknown dNTP. We find that the commonly used Klenow DNA polymerase may substitute the corresponding ribonucleotide for the unknown dNTP leading in some instances to a large overestimation of dNTPs. We now describe assay conditions for each dNTP that avoid ribonucleotide incorporation. For the dTTP and dATP assays it suffices to minimize the concentrations of the Klenow enzyme and of labeled dATP (or dTTP); for dCTP and dGTP we had to replace the Klenow enzyme with either the Taq DNA polymerase or Thermo Sequenase. We suggest that in some earlier reports ribonucleotide incorporation may have caused too high values for dGTP and dCTP.

摘要

真核细胞中四种脱氧核苷三磷酸(dNTP)的含量非常微小,仅能维持几分钟的 DNA 复制。单一 dNTP 的缺乏或过剩都会导致突变率增加、DNA 修复错误或线粒体 DNA 耗竭。通常通过酶促测定法来定量 dNTP,该方法中,DNA 聚合酶将放射性 dATP(或放射性 dTTP 在 dATP 测定法中)掺入到特定的合成寡核苷酸中,其掺入量与未知 dNTP 的浓度成正比。我们发现,常用的 Klenow DNA 聚合酶可能会用相应的核糖核苷酸替代未知的 dNTP,从而导致某些情况下对 dNTP 的严重高估。现在,我们为每种 dNTP 描述了避免核糖核苷酸掺入的测定条件。对于 dTTP 和 dATP 测定,只需将 Klenow 酶和标记的 dATP(或 dTTP)的浓度最小化即可;对于 dCTP 和 dGTP,我们必须用 Taq DNA 聚合酶或 Thermo Sequenase 取代 Klenow 酶。我们认为,在一些早期报告中,核糖核苷酸的掺入可能导致 dGTP 和 dCTP 的值过高。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7bb1/2847218/b1933f4e1537/gkp1141f1.jpg

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