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开发并验证了首个用于贝类提取物中海藻酸快速筛选的高性能侧向流免疫分析(HP-LFIA)。

Development and validation of the first high performance-lateral flow immunoassay (HP-LFIA) for the rapid screening of domoic acid from shellfish extracts.

机构信息

Neogen Europe Limited, The Dairy School, Auchincruive, Ayr, KA6 5HW, Scotland, UK; Institute for Global Food Security, School of Biological Sciences, Queen's University, David Keir Building, Stranmillis Road, Belfast BT9 5AG, UK.

出版信息

Talanta. 2013 Nov 15;116:663-9. doi: 10.1016/j.talanta.2013.07.027. Epub 2013 Jul 24.

Abstract

A lateral flow immunoassay (LFIA) has been developed and fully validated to detect the primary amnesic shellfish poisoning (ASP) toxin, domoic acid (DA). The performance characteristics of two versions of the test were investigated using spiked and naturally contaminated shellfish (mussels, scallops, oysters, clams, and cockles). The tests provide a qualitative result, to indicate the absence or presence of DA in extracts of shellfish tissues, at concentrations that are relevant to regulatory limits. The new rapid assay (LFIA version 2) was designed to overcome the performance limitations identified in the first version of the assay. The improved test uses an electronic reader to remove the subjective nature of the generated results, and the positive cut-off for screening of DA in shellfish was increased from 10 ppm (version 1) to 17.5 ppm (version 2). A simple extraction and test procedure was employed, which required minimal equipment and materials; results were available 15 min after sample preparation. Stability of the aqueous extracts at room temperature (22 °C) at four time points (up to 245 min after extraction) and across a range of DA concentrations was 100.3±1.3% and 98.8±2.4% for pre- and post-buffered extracts, respectively. The assay can be used both within laboratory settings and in remote locations. The accuracy of the new assay, to indicate negative results at or below 10 ppm DA, and positive results at or above 17.5 ppm, was 99.5% (n=216 tests). Validation data were obtained from a 2-day, randomised, blind study consisting of multiple LFIA lots (n=3), readers (n=3) and operators (n=3), carrying out multiple extractions of mussel tissue (n=3) at each concentration (0, 10, 17.5, and 20 ppm). No matrix effects were observed on the performance of the assay with different species (mussels, scallops, oysters, clams, and cockles). There was no impact on accuracy or interference from other phycotoxins, glutamic acid or glutamine with various strip incubations (8, 10, and 12 min). The accuracy of the assay, using naturally contaminated samples to indicate negative results at or below 12.5 ppm and positive results at or above 17.5 ppm, was 100%. Variability between three LFIA lots across a range of DA concentrations, expressed as coefficient of variation (% CV), was 1.1±0.4% (n=2 days) based on quantitative readings from the electronic reader. During an 8 week stability study, accuracy of the method with test strips stored at various temperatures (6, 22, 37 and 50 °C) was 100%. Validation for both versions included comparisons with results obtained using reference LC-UV methods.

摘要

已开发并充分验证了侧向流动免疫分析(LFIA),以检测原发性健忘贝类中毒(ASP)毒素,即软骨藻酸(DA)。使用经过污染和自然污染的贝类(贻贝、扇贝、牡蛎、蛤和鸟蛤)研究了两种测试版本的性能特征。该测试提供了定性结果,以指示贝类组织提取物中 DA 的存在或不存在,浓度与监管限制相关。新的快速检测(LFIA 版本 2)旨在克服检测中存在的性能限制。第一个版本的分析。改进后的测试使用电子读数器消除了生成结果的主观性,贝类中 DA 的筛查阳性截止值从 10 ppm(版本 1)提高到 17.5 ppm(版本 2)。采用了简单的提取和测试程序,仅需最少的设备和材料;在样品制备后 15 分钟即可获得结果。在室温(22°C)下,在四个时间点(提取后长达 245 分钟)和一系列 DA 浓度下,缓冲前和缓冲后提取物的稳定性分别为 100.3±1.3%和 98.8±2.4%。该检测既可以在实验室环境中使用,也可以在偏远地区使用。新检测的准确性为 99.5%(n=216 次测试),表明 DA 浓度低于或等于 10 ppm 时结果为阴性,DA 浓度高于或等于 17.5 ppm 时结果为阳性。验证数据是通过一项为期两天的随机、盲法研究获得的,该研究包括多个 LFIA 批次(n=3)、读数器(n=3)和操作员(n=3),对每个浓度(0、10、17.5 和 20 ppm)的贻贝组织进行多次提取。在使用不同物种(贻贝、扇贝、牡蛎、蛤和鸟蛤)时,未观察到对检测性能有任何基质效应。在各种条带孵育(8、10 和 12 分钟)中,未观察到其他藻毒素、谷氨酸或谷氨酰胺对准确性或干扰的影响。使用自然污染的样本,该检测在低于或等于 12.5 ppm 时结果为阴性,在高于或等于 17.5 ppm 时结果为阳性,其准确性为 100%。在 DA 浓度范围内,三种 LFIA 批次之间的变异性表示为变异系数(%CV),基于电子读数器的定量读数,为 1.1±0.4%(n=2 天)。在 8 周的稳定性研究中,在 6、22、37 和 50°C 下储存的测试条的方法准确性为 100%。两种版本的验证均包括与使用参考 LC-UV 方法获得的结果进行比较。

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