Non-competitive ELISA with broad specificity for microcystins and nodularins

Q3 Earth and Planetary Sciences Advances in Oceanography and Limnology Pub Date : 2017-05-03 DOI:10.4081/AIOL.2017.6349
S. Akter, M. Vehniäinen, J. Meriluoto, L. Spoof, U. Lamminmäki
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引用次数: 12

Abstract

Simple and cost-effective methods with sufficient sensitivities for preliminary screening of cyanobacterial toxins are in high demand for assessing water quality and safety. We have recently developed a highly sensitive and rapid time-resolved fluorometry based non-competitive immunoassay for detection of microcystins and nodularins. The assay is based on a synthetic broad-specific anti-immunocomplex antibody SA51D1 capable of recognizing the immunocomplex formed by a generic anti-Adda monoclonal antibody (mAb) bound to either microcystins or nodularins. Using the same antibody pair, here we describe a very simple and cost-efficient non-competitive ELISA test for microcystins and nodularins based on conventional alkaline phosphatase (AP) activity measurement. The recombinant SA51D1 single-chain fragment of antibody variable domain (scFv) was produced as a fusion with bacterial alkaline phosphatase in Escherichia coli . After one step affinity purification through His-tag, the scFv-AP fusion protein could directly be used in the assay. For the assay, toxin standard/sample, biotinylated anti-Adda mAb and the scFv-AP were incubated together for one hour on streptavidin-coated microtiter wells, washed and AP activity was then measured by incubating (1 h at 37 ˚C) with chromogenic substrate para-nitrophenylphosphate (pNPP). The assay was capable of detecting all the eleven tested toxin variants (microcystin-LR, -dmLR, -RR, -dmRR, -YR, LA -LY, -LF -LW, -WR, and nodularin-R) below WHO guide line value of 1 µg L -1 . The detection limit (based on blank+3SD response) for microcystin-LR was ~0.2 µg L -1 . The assay was verified using spiked (0.25 - 4 µg L -1 of microcystin-LR) tap, river and lake water samples with recoveries from 64 to 101%. The assay showed good correlation (r 2 >0.9) with four reference methods for its performance in detecting extracted intracellular microcystin/nodularin from 17 natural surface water samples. The described easy-to-perform assay has a high potential to be used in resource-poor settings as quantitative measurements can be obtained using a simple ELISA reader or easy-to-interpret qualitative results by visual readout. Based on the non-competitive format, the assay does not need any chemical toxin conjugates and offers robustness as compared to the currently available competitive format assays.
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对微囊藻毒素和结核蛋白具有广泛特异性的非竞争性ELISA
在评估水质和安全方面,对具有足够灵敏度的简单和成本效益的蓝藻毒素初步筛选方法的需求很高。我们最近开发了一种基于高灵敏度和快速时间分辨荧光法的非竞争免疫测定法,用于检测微囊藻毒素和结节藻毒素。该测定基于合成的宽特异性抗免疫复合物抗体SA51D1,其能够识别由与微囊藻毒素或结节藻毒素结合的通用抗Adda单克隆抗体(mAb)形成的免疫复合物。使用相同的抗体对,我们描述了一种基于传统碱性磷酸酶(AP)活性测量的微囊藻毒素和结节藻毒素的非常简单且成本效益高的非竞争性ELISA测试。在大肠杆菌中以与细菌碱性磷酸酶融合的方式制备了抗体可变结构域(scFv)的重组SA51D1单链片段。通过His-tag一步亲和纯化后,scFv-AP融合蛋白可直接用于测定。对于测定,将毒素标准品/样品、生物素化的抗Adda mAb和scFv AP在链霉亲和素包被的微量滴定孔上一起孵育1小时,洗涤,然后通过与显色底物对硝基苯基磷酸酯(pNPP)孵育(37˚C下孵育1 h)来测量AP活性。该测定法能够检测到低于世界卫生组织1µg L-1指导线值的所有11种测试毒素变体(微囊藻毒素-LR、-dmLR、-RR、-dmRR、-YR、LA-LY、-LF-LW、-WR和结瘤菌素-R)。微囊藻毒素LR的检测限(基于空白+3SD响应)为~0.2µg L-1。使用加标的(0.25-4µg L-1的微囊藻毒素LR)自来水、河流和湖泊样品验证了该测定,回收率为64%至101%。该方法对17份天然地表水样品中提取的细胞内微囊藻毒素/结节藻毒素的检测结果与四种参考方法具有良好的相关性(r2>0.9)。所描述的易于执行的测定具有在资源匮乏的环境中使用的高潜力,因为可以使用简单的ELISA读取器获得定量测量或通过视觉读出容易解释定性结果。基于非竞争性形式,该测定不需要任何化学毒素缀合物,并且与当前可用的竞争性形式测定相比具有稳健性。
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来源期刊
Advances in Oceanography and Limnology
Advances in Oceanography and Limnology Agricultural and Biological Sciences-Aquatic Science
CiteScore
2.00
自引率
0.00%
发文量
2
审稿时长
12 weeks
期刊介绍: Advances in Oceanography and Limnology was born in 2010 from the 35 years old Proceedings of the national congress of the Italian Association of Oceanology and Limnology. The AIOL Journal was funded as an interdisciplinary journal embracing both fundamental and applied Oceanographic and Limnological research, with focus on both single and multiple disciplines. Currently, two regular issues of the journal are published each year. In addition, Special Issues that focus on topics that are timely and of interest to a significant number of Limnologists and Oceanographers are also published. The journal, which is intended as an official publication of the AIOL, is also published in association with the EFFS (European Federation for Freshwater Sciences), which aims and objectives are directed towards the promotion of freshwater sciences throughout Europe. Starting from the 2015 issue, the AIOL Journal is published as an Open Access, peer-reviewed journal. Space is given to regular articles, review, short notes and opinion paper
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