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基于阳离子共轭聚合物荧光共振能量转移的荧光策略用于定量基因组 DNA 中的 5-(羟甲基)胞嘧啶。

Fluorescent strategy based on cationic conjugated polymer fluorescence resonance energy transfer for the quantification of 5-(hydroxymethyl)cytosine in genomic DNA.

机构信息

College of Chemistry and Molecular Sciences, Key Laboratory of Biomedical Polymers of Ministry of Education, Wuhan University , Wuhan, Hubei 430072, People's Republic of China.

出版信息

Anal Chem. 2013 Nov 19;85(22):10797-802. doi: 10.1021/ac4020676. Epub 2013 Oct 29.

DOI:10.1021/ac4020676
PMID:23991669
Abstract

DNA methylation is dynamically reprogrammed during early embryonic development in mammals. It can be explained partially by the discovery of 5-(hydroxymethyl)cytosine (5-hmC), 5-formylcytosine (5-fC), and 5-carboxylcytosine (5-caC), which are identified as key players involved in both active and passive demethylation pathways. As one of the ten-eleven translocation oxidation products, 5-hmC was found relatively abundant in neuron cells and embryonic stem cells. Herein we report a new method for 5-hmC quantification in genomic DNA based on CCP-FRET (cationic conjugated polymers act as the energy donor and induce fluorescence resonance energy transfer) assay combined with KRuO4 oxidation. 5-hmC in genomic DNA can be selectively transformed into 5-fC by the oxidation of KRuO4 and then labeled with hydroxylamine-BODIPY (BODIPY = 4,4-difluoro-4-bora-3a,4a-diaza-s-indacene) fluorophore through the reaction between 5-fC and hydroxylamine-BODIPY. After the fluorescently labeled DNA was captured by CCP through electrostatic interactions, a significant FRET between CCP and hydroxylamine-BODIPY fluorophore was observed. This CCP-FRET-based assay benefits from light-harvesting, large Stokes shift, and optical signal amplification properties of the CCP. Furthermore, this CCP-FRET-based assay was quite successfully demonstrated for the 5-hmC quantification in three types of cells (mESc, HeLa, HEK 293T), providing a much more convenient choice for 5-hmC quantification in genomic DNA.

摘要

DNA 甲基化在哺乳动物早期胚胎发育过程中被动态重编程。这可以部分归因于 5-(羟甲基)胞嘧啶 (5-hmC)、5-甲酰胞嘧啶 (5-fC) 和 5-羧基胞嘧啶 (5-caC) 的发现,它们被认为是参与主动和被动去甲基化途径的关键因素。作为十-十一易位氧化产物之一,5-hmC 在神经元细胞和胚胎干细胞中相对丰富。在此,我们报道了一种基于 CCP-FRET(阳离子共轭聚合物作为供体并诱导荧光共振能量转移)测定法结合 KRuO4 氧化的基因组 DNA 中 5-hmC 定量的新方法。KRuO4 的氧化可以将基因组 DNA 中的 5-hmC 选择性地转化为 5-fC,然后通过 5-fC 与羟胺-BODIPY(BODIPY=4,4-二氟-4-硼-3a,4a-二氮杂-s-茚)荧光团之间的反应进行标记。经氧化的 DNA 通过静电相互作用被 CCP 捕获后,CCP 与羟胺-BODIPY 荧光团之间观察到显著的 FRET。这种基于 CCP-FRET 的测定法得益于 CCP 的光捕获、大斯托克斯位移和光学信号放大特性。此外,该基于 CCP-FRET 的测定法在三种类型的细胞(mESc、HeLa、HEK 293T)中成功地用于 5-hmC 定量,为基因组 DNA 中 5-hmC 定量提供了更方便的选择。

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