Interlaboratory study on real-time PCR detection and quantification of the European anglerfish, pike, and seabream parvalbumin gene

IF 3 3区 农林科学 Q2 FOOD SCIENCE & TECHNOLOGY European Food Research and Technology Pub Date : 2024-05-21 DOI:10.1007/s00217-024-04578-w
Kamila Zdeňková, Subham Mukherjee, Marco A. Lopez Marin, Petra Horká, Veronika Kýrová, Miroslava Potůčková, Eliška Čermáková
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Abstract

This study presents a large-scale interlaboratory comparison (ILC) aimed at detecting and quantifying DNA from two European anglerfish (Lophius budegassa, Lophius piscatorius), pike (Esox lucius) and sea bream (Spondyliosoma cantharus) using real-time qPCR. To detect amplification of the parvalbumin genetic marker, single and multiplex qPCR assays using EvaGreen® dye or TaqMan™ probes were used. Genomic DNA isolated from target fish species and an advanced DNA calibrator, gBlocks® gene fragments, were used as standards. The DNA of anglerfish, pike and sea bream as well as their mixtures were analysed together with 14 other non-target fish species. All target fish samples were correctly identified by the participating laboratories. Qualitative assessment of anglerfish and seabream DNA showed an accuracy rate of 100%, while pike DNA achieved a match rate of 99%. Validation of quantitative protocols in four different laboratories consistently achieved z-scores below 2, indicating satisfactory performance and confirming the high degree of similarity of laboratory results. Furthermore, high accuracy and efficiency were demonstrated for the quantification of anglerfish and seabream DNA by triplex qPCR using TaqMan™ probes. Regarding the selected gene marker, the major fish allergenic protein parvalbumin enables indirect detection and quantification of the allergen in the sample. Therefore, the use of proposed protocols can significantly contribute to protecting the health of consumers and to controlling the food market.

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关于欧洲鮟鱇鱼、梭子鱼和鲷鱼副缬氨酸基因的实时 PCR 检测和定量的实验室间研究
本研究采用实时 qPCR 技术,对两种欧洲鮟鱇鱼(Lophius budegassa 和 Lophius piscatorius)、梭子鱼(Esox lucius)和海鲷(Spondyliosoma cantharus)的 DNA 进行了大规模实验室间比对。为了检测副卵磷脂基因标记的扩增,使用了 EvaGreen® 染料或 TaqMan™ 探针进行单倍和多倍 qPCR 检测。以从目标鱼种分离的基因组 DNA 和先进的 DNA 校准物 gBlocks® 基因片段为标准。鮟鱇鱼、梭子鱼、鲷鱼及其混合物的 DNA 与其他 14 种非目标鱼类一起进行了分析。参与实验室对所有目标鱼类样本都进行了正确鉴定。对鮟鱇鱼和鲷鱼 DNA 的定性评估显示准确率为 100%,而梭子鱼 DNA 的匹配率为 99%。四个不同实验室的定量方案验证的 Z 值始终低于 2,表明性能令人满意,并证实了实验室结果的高度相似性。此外,使用 TaqMan™ 探针进行三重 qPCR 对鮟鱇鱼和鲷鱼 DNA 进行定量分析的准确性和效率也很高。关于所选的基因标记,主要鱼类过敏原蛋白副缬白蛋白可间接检测和定量样品中的过敏原。因此,使用建议的方案可大大有助于保护消费者的健康和控制食品市场。
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来源期刊
European Food Research and Technology
European Food Research and Technology 工程技术-食品科技
CiteScore
6.60
自引率
3.00%
发文量
232
审稿时长
2.0 months
期刊介绍: The journal European Food Research and Technology publishes state-of-the-art research papers and review articles on fundamental and applied food research. The journal''s mission is the fast publication of high quality papers on front-line research, newest techniques and on developing trends in the following sections: -chemistry and biochemistry- technology and molecular biotechnology- nutritional chemistry and toxicology- analytical and sensory methodologies- food physics. Out of the scope of the journal are: - contributions which are not of international interest or do not have a substantial impact on food sciences, - submissions which comprise merely data collections, based on the use of routine analytical or bacteriological methods, - contributions reporting biological or functional effects without profound chemical and/or physical structure characterization of the compound(s) under research.
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