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首页> 外文期刊>The Analyst: The Analytical Journal of the Royal Society of Chemistry: A Monthly International Publication Dealing with All Branches of Analytical Chemistry >The mechanism and regularity of quenching the effect of bases on fluorophores: the base-quenched probe method
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The mechanism and regularity of quenching the effect of bases on fluorophores: the base-quenched probe method

机译:淬火碱对荧光团作用的机制和规律:碱淬火探针法

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The base-quenched probe method for detecting single nucleotide polymorphisms (SNPs) relies on realtime PCR and melting-curve analysis, which might require only one pair of primers and one probe. At present, it has been successfully applied to detect SNPs of multiple genes. However, the mechanism of the base-quenched probe method remains unclear. Therefore, we investigated the possible mechanism of fluorescence quenching by DNA bases in aqueous solution using spectroscopic techniques. It showed that the possible mechanism might be photo-induced electron transfer. We next analyzed electron transfer or transmission between DNA bases and fluorophores. The data suggested that in single-stranded DNA, the electrons of the fluorophore are transferred to the orbital of pyrimidine bases (thymine (T) and cytosine (C)), or that the electron orbitals of the fluorophore are occupied by electrons from purine bases (guanine (G) and adenine (A)), which lead to fluorescence quenching. In addition, the electrons of a fluorophore excited by light can be transmitted along double-stranded DNA, which gives rise to stronger fluorescence quenching. Furthermore, we demonstrated that the quenching efficiency of bases is in the order of G C = A = T and the capability of electron transmission of base-pairs in double-stranded DNA is in the order of CG = GC TA = AT (letters representing bases on the complementary strand of the probe are bold and underlined), and the most common commercial fluorophores including FAM, HEX, TET, JOE, and TAMRA could be influenced by bases and are in line with this mechanism and regularity.
机译:用于检测单个核苷酸多态性(SNP)的碱基淬火探针方法依赖于实时PCR和熔化曲线分析,这可能仅需要一对引物和一个探针。目前,它已成功应用于检测多种基因的SNP。然而,碱基淬火探针方法的机制仍不清楚。因此,我们研究了使用光谱技术通过DNA碱基在水溶液中的荧光猝灭机制。结果表明,可能的机制可能是光诱导的电子转移。我们接下来分析了DNA碱基和荧光团之间的电子转移或透射。该数据表明,在单链DNA中,荧光团的电子转移到嘧啶碱基(胸腺嘧啶(T)和胞嘧啶(C))中,或者荧光团的电子轨道被来自嘌呤碱的电子占据(鸟嘌呤(g)和腺嘌呤(a)),导致荧光猝灭。另外,通过光激发的荧光团的电子可以沿双链DNA传递,这导致荧光猝灭的较强。此外,我们证明碱基的淬火效率是G&GT的顺序。 C& = A& = T和双链DNA中碱对的电子传输的能力为CG& = GC> Ta& = AT(代表探针的互补链上的基础的字母是粗体和下划线的),以及包括FAM,HEX,TET,JOE和TAMRA的最常见的商业荧光团可能受到基础的影响,并符合这一点机制和规律性。

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