Dual-Mode Aptasensor Assembled by a WO3/Fe2O3 Heterojunction for Paper-Based Colorimetric Prediction/Photoelectrochemical Multicomponent Analysis

材料科学 适体 光电流 检出限 异质结 分析物 信号(编程语言) 脱氧核酶 生物传感器 光电子学 纳米技术 组合化学 计算机科学 化学 色谱法 遗传学 生物 程序设计语言
作者
Jianli Sun,Li Li,Shenguang Ge,Peini Zhao,Peihua Zhu,Mingliang Wang,Jinghua Yu
出处
期刊:ACS Applied Materials & Interfaces [American Chemical Society]
卷期号:13 (3): 3645-3652 被引量:46
标识
DOI:10.1021/acsami.0c19853
摘要

The programed bimodal photoelectrochemical (PEC)-sensing platform based on DNA structural switching induced by targets binding to aptamers was innovatively designed for the simultaneous detection of mucin 1 (MUC1) and microRNA 21 (miRNA-21). To promote excellent current intensity as well as enhance the sensitivity of aptasensors, the evenly distributed WO3/Fe2O3 heterojunction was prepared as a transducer material, notably reducing the background signal response and extending the absorption of light. The multifunctional paper-based biocathode was assembled to provide a visual colorimetric assay. When introducing the integrated signal probe (ISP) composed of signal probe 1 (sP1) and signal probe 2 (sP2) on paper-based working units modified with gold nanoparticles (AuNPs), recognition sites of two targets were formed. In the presence of MUC1 protein, both sP1 and the target on the working unit were released into the corresponding colorimetric unit because of the DNA specific recognition. The horseradish peroxidase–streptavidin (HRP–SA) carried by free sP1 could oxidize 3,3′,5,5′-tetramethylbenzidine (TMB) to turn a blue-colored oxidized TMB (oxTMB) in the presence of hydrogen peroxide (H2O2), which ultimately gained a higher photocurrent signal. Furthermore, miRNA-21 was modified on another working unit by binding with sP2, leading to changes in the current signal and thus enabling real-time detection of analytes with the assistance of a digital multimeter. The PEC aptasensor offered a wide dynamic range of 10 fg·mL–1–100 ng mL–1 for MUC1 and 0.1 pM–10 nM for miRNA-21, with a low detection limit of 3.4 fg·mL–1 and 36 fM, respectively. It laid the foundation for synchronous detection of multiple analytes and initiated a new way for the enhancement in modern next-generation disease diagnosis.
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