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多孔纳米酶:介孔氧化铁的过氧化物酶模拟活性用于比色法和电化学检测全基因组DNA甲基化

Porous nanozymes: the peroxidase-mimetic activity of mesoporous iron oxide for the colorimetric and electrochemical detection of global DNA methylation.

作者信息

Bhattacharjee Ripon, Tanaka Shunsuke, Moriam Sofia, Masud Mostafa Kamal, Lin Jianjian, Alshehri Saad M, Ahamad Tansir, Salunkhe Rahul R, Nguyen Nam-Trung, Yamauchi Yusuke, Hossain Md Shahriar A, Shiddiky Muhammad J A

机构信息

School of Environment and Science & Queensland Micro- and Nanotechnology Centre (QMNC), Griffith University, Nathan Campus, Nathan, QLD 4111, Australia.

出版信息

J Mater Chem B. 2018 Aug 7;6(29):4783-4791. doi: 10.1039/c8tb01132j. Epub 2018 Jul 6.

DOI:10.1039/c8tb01132j
PMID:32254305
Abstract

Nanomaterials (nanozymes) with peroxidase-mimetic activity have been widely used in biosensing platforms as low-cost, relatively stable and prevailing alternatives to natural enzymes. Herein, we report on the synthesis and application of the peroxidase-mimetic activity of mesoporous iron oxide (MIO) for the detection of global DNA methylation in colorectal cancer cell lines. The target DNA was extracted and denatured to get ssDNA followed by direct adsorption onto the surface of a bare screen-printed gold electrode (SPGE). A 5-methylcytosine antibody (5mC) functionalized nanomaterial (MIO-5mC) was then used to recognise the methylcytosine groups present on the SPGE. The MIO-5mC conjugates catalyse the TMB solution in the presence of hydrogen peroxide to give the colorimetric (i.e., naked-eye observation) and electrochemical detection of DNA methylation. The assay could successfully detect as low as 10% difference in the global DNA methylation level in synthetic samples and cell lines with good reproducibility and specificity (%RSD = <5%, for n = 3). This strategy avoids the use of natural enzyme horseradish peroxidase (HRP), traditional PCR based amplification and bisulfite treatment steps that are generally used in many conventional DNA methylation assays. We envisage that our assay could be a low-cost platform with great potential for genome-wide DNA methylation analysis in point-of-care applications.

摘要

具有过氧化物酶模拟活性的纳米材料(纳米酶)作为天然酶的低成本、相对稳定且普遍的替代品,已被广泛应用于生物传感平台。在此,我们报道了介孔氧化铁(MIO)的过氧化物酶模拟活性的合成及其在结肠癌细胞系中检测全基因组DNA甲基化的应用。提取目标DNA并使其变性以获得单链DNA,然后将其直接吸附到裸屏印刷金电极(SPGE)表面。接着使用5-甲基胞嘧啶抗体(5mC)功能化的纳米材料(MIO-5mC)来识别SPGE上存在的甲基胞嘧啶基团。MIO-5mC缀合物在过氧化氢存在下催化TMB溶液,从而实现DNA甲基化的比色法(即肉眼观察)和电化学检测。该测定法能够成功检测合成样品和细胞系中低至10%的全基因组DNA甲基化水平差异,具有良好的重现性和特异性(对于n = 3,%RSD = <5%)。该策略避免了使用天然酶辣根过氧化物酶(HRP)、许多传统DNA甲基化测定中通常使用的基于传统PCR的扩增和亚硫酸氢盐处理步骤。我们设想,我们的测定法可能是一个低成本平台,在即时护理应用中进行全基因组DNA甲基化分析具有巨大潜力。

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