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基于G-四链体/血红素DNAzyme的双扩增比率荧光ELISA,使用四面体DNA纳米结构作为支架用于超灵敏检测水生系统中的邻苯二甲酸二丁酯

Dual amplified ratiometric fluorescence ELISA based on G-quadruplex/hemin DNAzyme using tetrahedral DNA nanostructure as scaffold for ultrasensitive detection of dibutyl phthalate in aquatic system.

作者信息

Zhu Nuanfei, Li Xuesong, Liu Ye, Liu Jingfu, Wang Yawei, Wu Xiangyang, Zhang Zhen

机构信息

School of the Environment and Safety Engineering, Jiangsu University, Zhenjiang 212013, China; Department of Chemistry, University of Massachusetts, Amherst, MA 01003, United States.

School of the Environment and Safety Engineering, Jiangsu University, Zhenjiang 212013, China.

出版信息

Sci Total Environ. 2021 Aug 25;784:147212. doi: 10.1016/j.scitotenv.2021.147212. Epub 2021 Apr 21.

DOI:10.1016/j.scitotenv.2021.147212
PMID:33905933
Abstract

Dibutyl phthalate (DBP) is considered as one of the most widely used phthalate esters (PAEs), which has attracted worldwide concerns because of its potential threats to eco-environments and human health. Systematic investigations of DBP environmental occurrence contribute to the further risk assessment, which depends on effective and available analytical methods. In this study, an amplified ratiometric fluorescence ELISA was established for sensitive and high-throughput detection of DBP in the aquatic system based on a novel tetrahedral DNA nanostructure (TDN)-scaffolded-DNAzyme (Tetrazyme). Wherein, Tetrazyme was prepared by the precise folding of G-quadruplex sequence on three vertex angles of the TDN, together with hemin as the horseradish peroxidase (HRP)-mimicking enzyme. The rigid TDN avoided the local overcrowding effect to provide a reasonable spatial spacing on the interface for G-quadruplex sequence, increasing the collision chance between DNAzyme and substrates, improving the catalytic ability of DNAzyme effectively. Besides, streptavidin (SA) and biotin (bio) were used to anchor TDN and antibody, in which the specific binding of SA/bio could make more Tetrazyme conjugate on each signal element, resulting in the dual signal amplification. Meanwhile, the accuracy and precision were enhanced owing to the inherent built-in rectification to the environment from the dual output ratiometric fluorescence assay. Under the optimized conditions, the detection limit of this proposed method was 0.17 ng/mL (16 times lower than that of conventional ELISA using the same antibody) with a satisfactory accuracy (recoveries, 79.0%- 116.2%; CV, 2.1-6.5%). Overall, this platform provides a promising way for accurate, sensitive and rapid determination of DBP from environmental waters.

摘要

邻苯二甲酸二丁酯(DBP)被认为是使用最为广泛的邻苯二甲酸酯类(PAEs)之一,因其对生态环境和人类健康的潜在威胁而备受全球关注。对DBP在环境中的存在情况进行系统调查有助于进一步开展风险评估,而这依赖于有效且可行的分析方法。在本研究中,基于一种新型四面体DNA纳米结构(TDN)支架化DNA酶(四酶),建立了一种用于水生系统中DBP灵敏且高通量检测的扩增比率荧光酶联免疫吸附测定法。其中,四酶是通过在TDN的三个顶角上精确折叠G-四链体序列,并以血红素作为辣根过氧化物酶(HRP)模拟酶制备而成。刚性的TDN避免了局部拥挤效应,为G-四链体序列在界面上提供了合理的空间间距,增加了DNA酶与底物之间的碰撞机会,有效提高了DNA酶的催化能力。此外,链霉亲和素(SA)和生物素(bio)用于固定TDN和抗体,SA/bio的特异性结合可使更多的四酶结合在每个信号元件上,从而实现双信号放大。同时,由于双输出比率荧光测定法对环境的固有内置校正,提高了准确性和精密度。在优化条件下,该方法的检测限为0.17 ng/mL(比使用相同抗体的传统酶联免疫吸附测定法低16倍),具有令人满意的准确度(回收率为79.0%-116.2%;变异系数为2.1-6.5%)。总体而言,该平台为准确、灵敏且快速地测定环境水体中的DBP提供了一种有前景的方法。

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