Proximity hybridization induced rolling circle amplification for label-free SERS detection of the depression marker human apolipoprotein A4

化学 胶体金 检出限 滚动圆复制 DNA 载脂蛋白B 核酸 底漆(化妆品) 纳米颗粒 基质(水族馆) 吸附 组合化学 生物化学 色谱法 分子生物学 纳米技术 聚合酶 有机化学 胆固醇 材料科学 海洋学 地质学 生物
作者
Xianjiu Liao,Caiyi Zhang,Shang Qiu,Zhili Qiu,Qianli Tang,Shenyue Wu,Jie Xu,Biaoliang Wu,Zhao Liu,Fenglei Gao
出处
期刊:Talanta [Elsevier]
卷期号:244: 123402-123402 被引量:5
标识
DOI:10.1016/j.talanta.2022.123402
摘要

A new label-free method was developed for SERS detection of human apolipoprotein A4. Rolling circle amplification (RCA) was used, which could induce the production of AuNPs (poly adenine and adsorption gold nanoparticles). When there were two DNA labeled antibodies and target protein, MB1 (molecular beacon 1) was unfolded and the substrate was modified in the homogeneous solution, and the proximate complex was formed. The unfolded molecular beacon worked as a primer in the hybridization with the RCA template to start RCA, which could produce many long sequences of DNA containing amounts of adenines. The AuNPs were bound with the long-repeated adenine in the RCA product, causing accumulation of AuNPs on the surface of the electrode. It was indicated that the spectral characteristics of adenine at 736 cm-1 strongly dominated the SERS spectrum of DNA. Adenine worked as an internal marker for detecting human apolipoprotein A4 by using label-free SERS method. When the conditions were optimal, the detection of human apolipoprotein A4 was carried out from 10 pg mL-1 to 1000 ng mL-1, and the detection limit was low (4.1 pg mL-1). Meanwhile, the specificity was also excellent because the antibody could specifically bind with the corresponding antigen. In addition, since adenine was dominant in SERS spectra and the affinity between AuNPs and poly adenine was high, the detection procedure could be performed without any sophisticated modification. This method might provide a promising strategy for diagnosis in clinical practice.
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