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一种基于光活性聚合物的创新荧光生物分析策略,用于识别 DNA 甲基化:通过基因传感器技术研究 DNA 损伤的新平台。

An innovative fluorometric bioanalysis strategy towards recognition of DNA methylation using opto-active polymer: A new platform for DNA damage studies by genosensor technology.

机构信息

Department of Biology, Faculty of Natural Science, University of Tabriz, Tabriz, Iran.

Pharmaceutical Analysis Research Center, Tabriz University of Medical Sciences, Tabriz, Iran.

出版信息

J Mol Recognit. 2022 Nov;35(11):e2981. doi: 10.1002/jmr.2981. Epub 2022 Aug 15.

DOI:10.1002/jmr.2981
PMID:35767372
Abstract

Efficient pharmacotherapy of cancer is related to accurate recognition of genetic mutations and epigenetic alterations in the early-stage diagnosis. In the present study, a novel optical genosensor based on toluidine blue as photonic probe was developed to detection of DNA methylation using hybridization of pDNA with cDNA. Biomedical analysis was performed using UV-vis and fluorometric methods. For the first time, this strategy was applied for the distinction of methylated DNA from unmethylated-DNA-based on the interaction of optical probe with methylated-DNA and unmethylated DNA. Fluorescence spectroscopic data showed that poly-toluidine blue could be bind to DNA sequences and lead to different fluorescence patterns and could be used as an efficient geno-platform for the sensitive bioassay of mutation. The excitation and emission wavelengths were 580 and 630 nm, respectively. Non-binding of mismatch sequences with the optical probe was used as negative control. Under optimal conditions, linear range was 1 zM to 0.2 pm and the lower limit of quantitation was obtained as target concentrations ranging 1 zM. The designed genosensor showed high capability to distinct methylation from un-methylated. Therefore, the designed DNA-based bioassay could detect DNA methylation significantly. Finally, bioanalysis of real samples showed that the designed genosensor could use to detect DNA methylation which is a new platform for point of care analysis.

摘要

癌症的有效药物治疗与在早期诊断中准确识别基因突变和表观遗传改变有关。在本研究中,开发了一种基于甲苯胺蓝作为光子探针的新型光学生物传感器,用于使用 pDNA 与 cDNA 的杂交检测 DNA 甲基化。生物医学分析采用了紫外可见分光光度法和荧光分光光度法。首次应用该策略,基于光学探针与甲基化 DNA 和非甲基化 DNA 的相互作用,区分甲基化 DNA 与非甲基化 DNA。荧光光谱数据表明,聚甲苯胺蓝可以与 DNA 序列结合,导致不同的荧光模式,并可作为一种高效的基因平台,用于突变的灵敏生物测定。激发和发射波长分别为 580nm 和 630nm。非匹配序列与光学探针的非结合被用作阴性对照。在最佳条件下,线性范围为 1 nM 至 0.2 pm,检出限为 1 nM 左右。所设计的基因传感器表现出从非甲基化中区分甲基化的高能力。因此,所设计的基于 DNA 的生物测定法可以显著检测 DNA 甲基化。最后,对实际样品的生物分析表明,所设计的基因传感器可用于检测 DNA 甲基化,这是一种新的即时检测分析平台。

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