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基于适配体的微流控珠阵列传感器,采用多酶联纳米粒子扩增和量子点标记,用于同时检测多种分析物。

Aptamer-based microfluidic beads array sensor for simultaneous detection of multiple analytes employing multienzyme-linked nanoparticle amplification and quantum dots labels.

机构信息

School of Chemistry and Chemical Engineering, Hunan Institute of Engineering, Xiangtan 411104, People׳s Republic of China.

School of Chemistry and Chemical Engineering, Hunan Institute of Engineering, Xiangtan 411104, People׳s Republic of China.

出版信息

Biosens Bioelectron. 2014 Jul 15;57:22-9. doi: 10.1016/j.bios.2014.01.054. Epub 2014 Feb 5.

Abstract

This study reports the development of an aptamer-mediated microfluidic beads-based sensor for multiple analytes detection and quantification using multienzyme-linked nanoparticle amplification and quantum dots labels. Adenosine and cocaine were selected as the model analytes to validate the assay design based on strand displacement induced by target-aptamer complex. Microbeads functionalized with the aptamers and modified electron rich proteins were arrayed within a microfluidic channel and were connected with the horseradish peroxidases (HRP) and capture DNA probe derivative gold nanoparticles (AuNPs) via hybridization. The conformational transition of aptamer induced by target-aptamer complex contributes to the displacement of functionalized AuNPs and decreases the fluorescence signal of microbeads. In this approach, increased binding events of HRP on each nanosphere and enhanced mass transport capability inherent from microfluidics are integrated for enhancing the detection sensitivity of analytes. Based on the dual signal amplification strategy, the developed aptamer-based microfluidic bead array sensor could discriminate as low as 0.1 pM of adenosine and 0.5 pM cocaine, and showed a 500-fold increase in detection limit of adenosine compared to the off-chip test. The results proved the microfluidic-based method was a rapid and efficient system for aptamer-based targets assays (adenosine (0.1 pM) and cocaine (0.5 pM)), requiring only minimal (microliter) reagent use. This work demonstrated the successful application of aptamer-based microfluidic beads array sensor for detection of important molecules in biomedical fields.

摘要

本研究报告了一种基于适体的微流控珠传感器的开发,用于使用多酶连接的纳米颗粒扩增和量子点标记物对多种分析物进行检测和定量。选择腺苷和可卡因作为模型分析物,基于目标-适体复合物诱导的链置换验证基于微流控的分析物设计。功能化有适体的微珠和修饰的富电子蛋白被排列在微流道内,并通过杂交与辣根过氧化物酶(HRP)和捕获 DNA 探针衍生的金纳米颗粒(AuNPs)连接。目标-适体复合物诱导的适体构象转换导致功能化 AuNPs 的位移,并降低微珠的荧光信号。在这种方法中,每个纳米球上 HRP 的结合事件增加和微流控固有的增强质量传输能力被集成用于增强分析物的检测灵敏度。基于双信号放大策略,开发的基于适体的微流控珠阵列传感器能够区分低至 0.1 pM 的腺苷和 0.5 pM 的可卡因,与芯片外测试相比,腺苷的检测限提高了 500 倍。结果证明基于微流控的方法是一种快速有效的基于适体的靶标分析(腺苷(0.1 pM)和可卡因(0.5 pM))的系统,仅需要最小(微升)的试剂用量。这项工作证明了基于适体的微流控珠阵列传感器在生物医学领域重要分子检测中的成功应用。

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