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基于肉眼观察的免疫层析半定量分析策略。

A naked-eye based strategy for semiquantitative immunochromatographic assay.

机构信息

Oil Crops Research Institute, Chinese Academy of Agricultural Sciences, Wuhan 430062, China.

出版信息

Anal Chim Acta. 2012 Aug 31;740:74-9. doi: 10.1016/j.aca.2012.06.015. Epub 2012 Jun 17.

DOI:10.1016/j.aca.2012.06.015
PMID:22840653
Abstract

It is critical to develop a cost-effective quantitative/semiquantitative assay for rapid diagnosis and on-site detection of toxic or harmful substances. Here, a naked-eye based semiquantitative immunochromatographic strip (NSI-strip) was developed, on which three test lines (TLs, TL-I, TL-II and TL-III) were dispensed on a nitrocellulose membrane to form the test zone. Similar as the traditional strip assay for small molecule, the NSI-strip assay was also based on the competitive theory, difference was that the analyte competed three times with the capture reagent for the limited number of antibody binding sites. After the assay, the number of TLs developed in the test zone was inversely proportional to the analyte concentration, thus analyte content levels could be determined by observing the appeared number of TLs. Taking aflatoxin B(1) as the model analyte, visual detection limit of the NSI-strip was 0.06 ng mL(-1) and threshold concentrations for TL-I-III were 0.125, 0.5, and 2.0 ng mL(-1), respectively. Therefore, according to the appeared number of TLs, the following concentration ranges would be detectable by visual examination: 0-0.06 ng mL(-1) (negative samples), and 0.06-0.125 ng mL(-1), 0.125-0.5 ng mL(-1), 0.5-2.0 ng mL(-1) and >2.0 ng mL(-1) (positive samples). That was to say, compared to traditional strips the NSI-strip could offer more parameter information of the target analyte content. In this way, the NSI-strip improved the qualitative presence/absence detection of traditional strips by measuring the content (range) of target analytes semiquantitatively.

摘要

开发一种经济有效的定量/半定量分析方法,用于快速诊断和现场检测有毒或有害物质至关重要。在此,开发了一种基于肉眼的半定量免疫层析条(NSI 条),在硝酸纤维素膜上分配了三条测试线(TLs,TL-I,TL-II 和 TL-III)以形成测试区。与小分子的传统条带分析类似,NSI 条带分析也基于竞争理论,不同之处在于分析物与捕获试剂竞争三次以获得有限数量的抗体结合位点。分析完成后,测试区中形成的 TL 数量与分析物浓度成反比,因此可以通过观察 TL 出现的数量来确定分析物含量水平。以黄曲霉毒素 B(1)为模型分析物,NSI 条的目视检测限为 0.06ngmL(-1),TL-I-III 的阈值浓度分别为 0.125、0.5 和 2.0ngmL(-1)。因此,根据 TL 的出现数量,通过目视检查可以检测到以下浓度范围:0-0.06ngmL(-1)(阴性样品)和 0.06-0.125ngmL(-1)、0.125-0.5ngmL(-1)、0.5-2.0ngmL(-1)和>2.0ngmL(-1)(阳性样品)。也就是说,与传统条带相比,NSI 条带可以通过半定量测量目标分析物含量提供更多的目标分析物含量信息。这样,NSI 条带通过半定量测量目标分析物的含量(范围)来提高传统条带的定性存在/不存在检测。

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