Simultaneous detection and quantification of two European anglerfishes by novel genomic primer

被引:9
|
作者
Mukherjee, Subham [1 ,2 ]
Hanak, Petr [2 ]
Jilkova, Diliara [2 ,3 ]
Musilova, Zuzana [4 ]
Horka, Petra [1 ]
Lerch, Zdenek [2 ,4 ]
Zdenkova, Kamila [3 ]
Cermakova, Eliska [2 ,3 ]
机构
[1] Charles Univ Prague, Inst Environm Studies, Fac Sci, Benatska 2, Prague 2, Czech Republic
[2] Food Res Inst Prague, Dept Chem Biochem & Food Microbiol, Radiova 1285-7, Prague 10, Czech Republic
[3] Univ Chem & Technol Prague, Dept Biochem & Microbiol, Tech 5, Prague 6, Czech Republic
[4] Charles Univ Prague, Fac Sci, Dept Zool, Vinicna 7, Prague 2, Czech Republic
关键词
Anglerfish; Adulteration; Fish identification; Food frauds; Genetic marker; Lophius; Parvalbumin; PCR sequencing; REAL-TIME PCR; MAJOR ALLERGEN PARVALBUMIN; LOPHIUS-BUDEGASSA; RAPID DETECTION; FISH ALLERGEN; RFLP-ANALYSIS; CYTOCHROME-B; 2ND INTRON; IDENTIFICATION; AUTHENTICATION;
D O I
10.1016/j.jfca.2022.104992
中图分类号
O69 [应用化学];
学科分类号
081704 ;
摘要
Globalisation has led to increased trade and consumption of fish worldwide. As international trade and con-sumption of fish increases, so does the likelihood of fish being adulterated. It is often an illegal exchange of species where a cheaper species is substituted for a more expensive and rarer one. In Europe, the anglerfish (Lophius piscatorius) is often traded as the rarer, more popular black-bellied anglerfish (Lophius budegassa). To improve our ability to monitor and detect adulterants in these fish species, we developed a real-time PCR assay that allows for the simultaneous detection and quantification of L. piscatorius and L. budegassa. The newly designed primers target the second intron of the genomic gene parvalbumin. The proposed methodology shows good robustness, efficiency and high specificity. Of the 47 species tested, only Lophius species were amplified. Their differentiation is possible by analysing melting curves with an average Tm of 70.1 degrees C for L. piscatorius and 75.3 degrees C for L. budegassa, respectively. The detection limit for both species was 0.050 ng/mu l. The assay also provides a tool to quantify parvalbumin in European anglerfish. The findings point to the use of the method proposed as a potential tool in forensic investigations to prevent illegal species substitutions, mislabeling, and food fraud.
引用
收藏
页数:9
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