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Chimeric RNA-DNA Molecular Beacons for Quantification of Nucleic Acids, Single Nucleotide Polymophisms, and Nucleic Acid Damage

机译:用于定量核酸,单核苷酸多态性和核酸损伤的嵌合RNA-DNA分子信标

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摘要

Single nucleotide polymorphisms (SNPs) are the main cause for variations in the human genome. DNA lesions, such as cyclobutane pyrimidine dimers (CPDs), [6-4] pyrimidine-pyrimidinones, dewar pyrimidinones, and photo-hydrates, can subsequently lead to mutagenesis, carcinogenesis, and cell death. Much effort has focused on methods for detecting DNA, SNPs, or damaged nucleic acids. However, almost all of the proposed methods consist of multistep procedures, are limited to specific types of damage, some of these methods require expensive instruments, and some suffer from a high level of interferences. In this paper, we present a novel, simple, mix-and-read assay for the detection of nucleic acids that is general for all types of SNPs and nucleic acid damage. This method uses a chimeric RNA-DNA molecular beacon (chMB). The calibration curve of the chMB for detecting single base mismatch and ultraviolet (UV)-induced DNA damage shows good linearity (R~2 = 0.981 and 0.996, respectively) and limits of detection of 10.4 ± 2.2 and 8.64 ± 1.2 nM, respectively. The chimeric RNA-DNA MB proves to be a more sensitive and selective tool for the quantification of nucleic acids, DNA mismatches, and UV-induced DNA damage than DNA MBs.
机译:单核苷酸多态性(SNP)是人类基因组变异的主要原因。 DNA损伤,例如环丁烷嘧啶二聚体(CPD),[6-4]嘧啶-嘧啶酮,杜瓦嘧啶酮和光合水合物,可随后导致诱变,致癌作用和细胞死亡。许多努力集中在检测DNA,SNP或受损核酸的方法上。但是,几乎所有提议的方法都由多步骤程序组成,仅限于特定类型的损坏,其中一些方法需要昂贵的仪器,而另一些方法则受到严重干扰。在本文中,我们提出了一种新颖,简单,混合阅读的检测核酸的检测方法,该检测方法适用于所有类型的SNP和核酸损伤。此方法使用嵌合RNA-DNA分子信标(chMB)。用于检测单碱基错配和紫外线(UV)诱导的DNA损伤的chMB的校准曲线显示出良好的线性(分别为R〜2 = 0.981和0.996),检出限分别为10.4±2.2和8.64±1.2 nM。与DNA MBs相比,嵌合RNA-DNA MB被证明是用于定量核酸,DNA错配和紫外线诱导的DNA损伤的更灵敏和更具选择性的工具。

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