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电化学适体传感器利用三丙胺氧化来探测目标和互补核苷酸之间的分子内位移,用于蛋白质阵列。

Electrochemical aptasensor using the tripropylamine oxidation to probe intramolecular displacement between target and complementary nucleotide for protein array.

机构信息

Research Center for Analytical Sciences, College of Chemistry, Nankai University, 94 Weijin Road, Tianjin 300071, China.

出版信息

Biosens Bioelectron. 2011 Feb 15;26(6):2905-10. doi: 10.1016/j.bios.2010.11.035. Epub 2010 Dec 1.

DOI:10.1016/j.bios.2010.11.035
PMID:21183329
Abstract

Tripropylamine (TPA) has different oxidation efficiency at double stranded (ds)-and single stranded (ss)-DNA-modified electrodes. Using this property, a simple but sensitive biosensor using TPA oxidation to probe the intramolecular displacement was constructed with the analysis of lysozyme as model for the first time. After the complementary ss-DNA strand of anti-lysozyme aptamer was immobilized onto gold electrode via gold-thiol bond, the incubation with the aptamer resulted in the formation of ds-DNA. Lysozyme (in 10 μL sample) binding with aptamer displaced the complementary strand because of the high affinity of lysozyme and its aptamer, corresponding to the dissociation of the ds-DNA. The modified electrode was swept in 20mM TPA solution from 0.2 to 0.95 V. The difference in oxidation current was used to quantify the content of lysozyme with a linear range from 1.0 pM to 1.1 nM. That means 10 amol or 6.0 × 10(6) lysozyme molecules can be detected. Because the signal is produced from the preconcentrated TPA at the electrode surface, the high sensitivity is achieved over the single site labelling strategy. The proposed method is simple, stable, specific, and time-saving while the complicated sample pre-treatment and the labelling to the DNA strand are avoided. The biosensor was validated by the analysis of the diluted egg white sample directly. The recovery and reproducibility were 93.3-100% and 1.4-4.2%, respectively.

摘要

三亚丙胺(TPA)在双链(ds)和单链(ss)DNA 修饰电极上具有不同的氧化效率。利用这一特性,首次构建了一种简单但灵敏的生物传感器,该传感器利用 TPA 氧化来探测分子内位移,以溶菌酶为模型进行分析。将抗溶菌酶适体的互补 ss-DNA 链通过金-硫键固定在金电极上后,与适体孵育会形成 ds-DNA。由于溶菌酶与其适体的高亲和力,溶菌酶(在 10 μL 样品中)与适体结合会取代互补链,从而导致 ds-DNA 解离。将修饰后的电极在 20mM TPA 溶液中从 0.2 到 0.95V 进行扫速。氧化电流的差异用于定量测定溶菌酶的含量,线性范围为 1.0 pM 至 1.1 nM。这意味着可以检测到 10 amol 或 6.0×10(6)个溶菌酶分子。由于信号是由电极表面预浓缩的 TPA 产生的,因此与单个位点标记策略相比,实现了高灵敏度。该方法简单、稳定、特异,且节省时间,同时避免了复杂的样品预处理和 DNA 链标记。通过直接分析稀释的蛋清样品验证了该生物传感器的性能。回收率和重现性分别为 93.3-100%和 1.4-4.2%。

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