DNA-based authentication for insect-based feedstuffs: The case study of Tenebrio molitor and Hermetia illucens

被引:0
作者
Filipa-Silva, Andreia [1 ]
Martins, Thaise [1 ,2 ]
Mota, Maria J. [3 ,4 ]
Almeida, Andre [5 ,6 ]
Murta, Daniel [7 ,8 ]
Valente, Luisa M. P. [1 ,2 ]
Gomes, Sonia [1 ,2 ]
机构
[1] Univ Porto, Ctr Interdisciplinar Invest Marinha & Ambiental, CIIMAR CIMAR LA, Ave Gen Norton de Matos S-N, P-4450208 Matosinhos, Portugal
[2] Univ Porto, ICBAS, Inst Ciencias Biomed Abel Salazar, Rua Jorge Viterbo Ferreiro 228, P-4050313 Porto, Portugal
[3] Soc Oleos & Racoes SA, SORGAL, Estr Nacl 109, P-3880728 S Joao De Ovar, Portugal
[4] SAVINOR Soc Avicola Norte SA, Rua Cancela Vermelha 450, P-4785011 Trofa, Portugal
[5] Comercio & Ind Sebo SA, SEBOL, Rua Padre Adriano 61, P-2660119 Loures, Portugal
[6] Ind Transformadora Subprod SA, ITS, Rua Fabr 53, P-2100406 Coruche, Portugal
[7] Ingredient Odyssey SA, Thunder Foods Lda, Rua Comendador Jose Julio Eloy,Lote 7-A, P-2005332 Santarem, Portugal
[8] Ingredient Odyssey SA, EntoGreen, Rua Cidade Santarem 140, P-2005079 Santarem, Portugal
关键词
Tenebrio molitor; Hermetia illucens; Novel Protein Sources; Species Identification; Real-time PCR; Food Safety; Insect Authentication; REAL-TIME PCR;
D O I
10.1016/j.jfca.2024.107175
中图分类号
O69 [应用化学];
学科分类号
081704 ;
摘要
The rising demand for new protein sources increases the risk of fraud, particularly through misleading labelling, that can pose biosecurity hazards, such as allergic reactions in sensitised individuals. Ensuring authenticity of insect-based feed and food items is a top priority within the European Union. Addressing this need, this study developed two qPCR assays for insect species-specific detection/quantification in commercial meals, hydrolysates, and various animal feed products. These methods differentiated and quantified Tenebrio molitor (yellow mealworm) and Hermetia illucens (black soldier fly), enabling the authentication of various commercial feed and food matrices. qPCR targeting cytochrome b gene of T. molitor and NADH dehydrogenase gene of H. illucens detected DNA concentrations as low as 2 pg/mu L for T. molitor and 0.2 pg/mu L for H. illucens, identifying these insects in mixtures down to 0.24 % of inclusion in aquaculture feed. Additionally, both qPCR assays share the same thermal cycling conditions, enabling to detect T. molitor and H. illucens in a single run. In conclusion, this study demonstrates that these methods have strong analytical performance, confirming their suitability across complex matrices in food and feed applications. The qPCR offers a rapid, cost-effective tool for verifying EFSAauthorized insects in EU supply chains, from production to consumption.
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页数:8
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