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一种无 G-四链体/血红素结构损伤的方法,用于抑制过氧化物酶模拟 DNA 酶活性,从而开发用于生物传感的方法。

A G-quadruplex/hemin structure-undamaged method to inhibit peroxidase-mimic DNAzyme activity for biosensing development.

机构信息

Hunan Province Key Laboratory of Edible Forestry Resources Safety and Processing Utilization, National Engineering Laboratory for Deep Process of Rice and Byproducts, Central South University of Forestry and Technology, Changsha, 410004, PR China.

Research and Development of Center, China Tobacco Yunnan Industrial Co., Ltd., Kunming, 650231, China.

出版信息

Anal Chim Acta. 2022 Aug 15;1221:340143. doi: 10.1016/j.aca.2022.340143. Epub 2022 Jul 6.

DOI:10.1016/j.aca.2022.340143
PMID:35934375
Abstract

Damaging the structure of the G-quadruplex (G4) to prevent the formation of the G4/hemin complex is presently the only available method to inhibit the activity of the peroxidase-mimic DNAzyme. In this study, a unique intramolecular inhibitory effect of the adjacent base-pair (InE(N:N)), by installing a rationally adjacent base-pair of the G4 core sequence, is proposed for the inhibition of the DNAzyme activity, which eliminates the need to damage the entire G4 structure. Various base pairs show different abilities to inhibit DNAzyme activity. The adjacent adenine: thymine pair possesses the best inhibitory efficiency (17 times). Through detailed investigations of the InE(N:N), it was revealed that the adjacent adenine: thymine pair downregulated the formation of compound I in the catalytic process, thus inhibiting the G4 DNAzyme activity. The mechanism of inhibition indicated that the carbonyl group on the hexatomic ring of the complementary base played an important role. To further reflect the advantages of the proposed strategy, two InE(N:N)-based biosensors were developed for DNA analysis and Uracil-DNA glycosylase (UDG) detection. Compared with existing DNAzyme-based methods, the application of InE(N: N) facilitates the real-time assay and simplifies the design difficulty. Therefore, InE(N:N) provides new insights into the regulation of the DNAzyme activity and offers an efficient approach for the future application of DNAzyme.

摘要

破坏 G-四链体 (G4) 的结构以阻止 G4/血红素复合物的形成是目前抑制过氧化物酶模拟 DNA 酶活性的唯一可用方法。在这项研究中,通过在 G4 核心序列的合理相邻碱基对中安装相邻碱基对(InE(N:N)),提出了一种独特的分子内抑制效应(InE(N:N)),用于抑制 DNA 酶活性,从而无需破坏整个 G4 结构。各种碱基对显示出不同的抑制 DNA 酶活性的能力。相邻的腺嘌呤:胸腺嘧啶对具有最佳的抑制效率(17 倍)。通过对 InE(N:N)的详细研究,揭示了相邻的腺嘌呤:胸腺嘧啶对在催化过程中下调了化合物 I 的形成,从而抑制了 G4 DNA 酶活性。抑制机制表明,互补碱基的六元环上的羰基基团起重要作用。为了进一步反映所提出策略的优势,开发了两种基于 InE(N:N)的生物传感器用于 DNA 分析和尿嘧啶-DNA 糖基化酶 (UDG) 检测。与现有的 DNA 酶基方法相比,InE(N:N)的应用促进了实时分析,并简化了设计难度。因此,InE(N:N)为 DNA 酶活性的调节提供了新的见解,并为 DNA 酶的未来应用提供了一种有效的方法。

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