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基于发夹 DNA 探针修饰的金纳米粒子和杂交链式反应辅助放大的庆大霉素比色聚集分析检测法。

Colorimetric aggregation assay for kanamycin using gold nanoparticles modified with hairpin DNA probes and hybridization chain reaction-assisted amplification.

机构信息

School of Biosystems Engineering and Food Science, Zhejiang University, Hangzhou, 310058, People's Republic of China.

Zhejiang A&F University, Hangzhou, 311300, People's Republic of China.

出版信息

Mikrochim Acta. 2019 Jun 13;186(7):448. doi: 10.1007/s00604-019-3574-7.

DOI:10.1007/s00604-019-3574-7
PMID:31197488
Abstract

The authors describe a colorimetric method for determination of kanamycin by using gold nanoparticles (AuNPs) as the element of signal-conversion and by applying hybridization chain reaction-assisted signal amplification. The assay is carried out by monitoring the absorbance change and color change adding salt to the reaction solution containing kanamycin (analyte), hairpin DNA probe, and AuNPs. Three hairpin DNA probes with sticky ends were absorbed on the AuNPs via their sticky ends. Cating with DNA prevents them from salt-induced aggregation (which leads to a color change from red to blue) in the complete absence of kanamycin. In contrast, in the presence of kanamycin, the aptamer hairpin DNA probe binds kanamycin, and the newly exposed section of DNA triggers a cascade of hybridization chain reactions with formation of numerous dsDNAs. On addition of salt, the AuNPs form blue aggregates due to the repulsion between dsDNA and AuNPs. Under optimal conditions, the ration of absorbance at 520 and 630 nm drops with the kanamycin concentration in the range from 1 to 40 μM, and the limit of detection is 0.68 μM. The assay can selectively distinguish kanamycin from other antibiotics. The method was applied to kanamycin detection in (spiked) milk samples and gave excellent recoveries. Graphical abstract Schematic presentation of colorimetric method for kanamycin detection using gold nanoparticles modified with hairpin DNA probes and hybridization chain reaction-assisted amplification.

摘要

作者描述了一种通过金纳米粒子(AuNPs)作为信号转换元件,并应用杂交链式反应辅助信号放大来测定卡那霉素的比色法。该测定法通过监测添加盐到含有卡那霉素(分析物)、发夹 DNA 探针和 AuNPs 的反应溶液中引起的吸光度变化和颜色变化来进行。带有粘性末端的三个发夹 DNA 探针通过其粘性末端被吸附在 AuNPs 上。在没有卡那霉素的情况下,DNA 加帽可防止它们因盐诱导的聚集(导致颜色从红色变为蓝色)。相比之下,在存在卡那霉素的情况下,适体发夹 DNA 探针与卡那霉素结合,新暴露的 DNA 部分触发了一系列杂交链式反应,形成了许多 dsDNA。加入盐后,由于 dsDNA 和 AuNPs 之间的排斥作用,AuNPs 形成蓝色聚集体。在最佳条件下,520nm 和 630nm 处的吸光度比值随卡那霉素浓度在 1 至 40μM 范围内下降,检测限为 0.68μM。该测定法可以选择性地区分卡那霉素与其他抗生素。该方法已应用于(添加)牛奶样品中的卡那霉素检测,并给出了良好的回收率。

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