Gold nanoparticle/MXene for multiple and sensitive detection of oncomiRs based on synergetic signal amplification

生物传感器 检出限 滚动圆复制 纳米技术 线性范围 核酸酶 材料科学 胶体金 电极 纳米颗粒 化学 色谱法 DNA 聚合酶 生物化学 物理化学
作者
Mohsen Mohammadniaei,Aneesh Koyappayil,Yi Sun,Junhong Min,Minho Lee
出处
期刊:Biosensors and Bioelectronics [Elsevier]
卷期号:159: 112208-112208 被引量:88
标识
DOI:10.1016/j.bios.2020.112208
摘要

Multiple and sensitive detection of oncomiRs for accurate cancer diagnostics is still a challenge. Here, a synergetic amplification strategy was introduced by combining a MXene-based electrochemical signal amplification and a duplex-specific nuclease (DSN)-based amplification system for rapid, attomolar and concurrent quantification of multiple microRNAs on a single platform in total plasma. Synthesized MXene-Ti3C2Tx modified with 5 nm gold nanoparticles (AuNPs) was casted on a dual screen-printed gold electrode to host vast numbers of DNA probes identically co-immobilized on dedicated electrodes. Interestingly, presence of MXene provided biofouling resistance and enhanced the electrochemical signals by almost 4 folds of magnitude, attributed to its specious surface area and remarkable charge mobility. The 5 nm AuNPs were perfectly distributed within the whole flaky architect of the MXene to give rise to the electrochemical performance of MXene and provide the thiol-Au bonding feature. This synergetic strategy reduced the DSN-based biosensors' assay time to 80 min, provided multiplexability, antifouling activity, substantial sensitivity and specificity (single mutation recognition). The limit of detection of the proposed biosensor for microRNA-21 and microRNA-141 was respectively 204 aM and 138 aM with a wide linear range from 500 aM to 50 nM. As a proof of concept, this newly-developed strategy was coupled with a 96-well adaptive sensing device to successfully profile three cancer plasma samples based on their altered oncomiR abundances.
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