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商用血糖仪作为信号转换器,用于简单评估 DNA 甲基转移酶活性和抑制剂筛选。

Commercial glucometer as signal transducer for simple evaluation of DNA methyltransferase activity and inhibitors screening.

机构信息

College of Chemistry and Environmental Engineering, Yangtze University, Jingzhou 434023, PR China.

College of Chemistry and Environmental Engineering, Yangtze University, Jingzhou 434023, PR China.

出版信息

Anal Chim Acta. 2018 Feb 25;1001:18-23. doi: 10.1016/j.aca.2017.11.045. Epub 2017 Nov 23.

DOI:10.1016/j.aca.2017.11.045
PMID:29291802
Abstract

DNA methyltransferase (MTase) plays an important role in many biological processes and has been recognized as a predictive cancer biomarker far before other signs of malignancy and a therapeutic target in cancer treatment. Thus simple and sensitive determination of DNA MTase activity is urgently required. The commercially available glucometer is considered as the most successful point-of-care (POC) sensor up to date, and researchers extend its application in monitoring different types of targets rather than only glucose. Here, we developed a simple strategy for the sensitive detection of the DNA MTase (using M.SssI as an example) activity by using a glucometer as the signal transducer. A S1/S2 hybrid probe was designed including a specific recognition sequence for both DNA MTase and restriction endonuclease, and a complementary sequence for biotin-S3. Firstly, the S1/S2 hybrid probe was self-assembled on the gold electrode and methylated by M.SssI MTase to form the methylated dsDNA. Then, HpaII endonuclease specifically cleaved the residue of the unmethylated dsDNA. Subsequently, biotin-S3 hybridized with the overhang sequence of the methylated dsDNA. Finally, the biotin tag was successively combined with streptavidin (STV) and biotin-invertase. The invertase efficiently catalyzed the hydrolysis of sucrose to generate abundant glucose, which led to an amplified response of glucometer. This strategy could detect DNA MTase activity as low as 0.3 U mL with good selectivity against other two cytosine MTases (HaeIII MTase and AluI MTase), and be successfully applied for screening the DNA MTase inhibitors (5-azacytidine and 5-aza-2'-deoxycytidine), implying our proposed method holds great promising application in early cancer diagnosis and therapeutics.

摘要

DNA 甲基转移酶 (MTase) 在许多生物过程中发挥着重要作用,它作为一种预测癌症的生物标志物,在其他恶性肿瘤的迹象和癌症治疗的治疗靶点出现之前就已经被认识到。因此,迫切需要简单、灵敏地测定 DNA MTase 活性。目前,市售的血糖仪被认为是最成功的即时检测(POC)传感器之一,研究人员将其应用扩展到监测不同类型的靶标,而不仅仅是葡萄糖。在这里,我们开发了一种简单的策略,利用血糖仪作为信号转换器,灵敏地检测 DNA MTase(以 M.SssI 为例)的活性。设计了一种 S1/S2 杂交探针,它包含了 DNA MTase 和限制内切酶的特异性识别序列,以及生物素-S3 的互补序列。首先,S1/S2 杂交探针在金电极上自组装,并被 M.SssI MTase 甲基化,形成甲基化的 dsDNA。然后,HpaII 内切酶特异性地切割未甲基化 dsDNA 的残留部分。随后,生物素-S3 与甲基化 dsDNA 的突出序列杂交。最后,生物素标签与链霉亲和素(STV)和生物素-蔗糖酶相继结合。蔗糖酶有效地催化蔗糖水解生成大量的葡萄糖,从而使血糖仪的响应得到放大。该策略可检测低至 0.3 U mL 的 DNA MTase 活性,对其他两种胞嘧啶 MTase(HaeIII MTase 和 AluI MTase)具有良好的选择性,并成功应用于筛选 DNA MTase 抑制剂(5-氮杂胞苷和 5-氮杂-2'-脱氧胞苷),这表明我们提出的方法在癌症早期诊断和治疗中有很大的应用前景。

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