A Rapid Method for the Identification of Fresh and Processed Pagellus erythrinus Species against Frauds

被引:15
作者
Ceruso, Marina [1 ]
Mascolo, Celestina [1 ,2 ]
De Luca, Pasquale [3 ]
Venuti, Iolanda [1 ]
Smaldone, Giorgio [4 ]
Biffali, Elio [3 ]
Anastasio, Aniello [1 ]
Pepe, Tiziana [1 ]
Sordino, Paolo [2 ]
机构
[1] Univ Naples Federico II, Dept Vet Med & Anim Prod, Via F Delpino 1, I-80137 Naples, Italy
[2] Stn Zool Anton Dohrn, Dept Biol & Evolut Marine Organisms, I-80121 Naples, Italy
[3] Stn Zool Anton Dohrn, Dept Res Infrastruct Marine Biol Resources, I-80121 Naples, Italy
[4] Univ Naples Federico II, Dept Agr Sci, Via Univ 100, I-80055 Naples, Italy
关键词
fish species authentication; mtDNA; mitogenomics; common pandora; Pagellus erythrinus; Sparidae; COMPLETE MITOCHONDRIAL GENOME; DNA SEQUENCE; FAMILY SPARIDAE; PERCIFORMES; SEABREAM; DENTEX; PHYLOGENIES; MARKERS; PCR;
D O I
10.3390/foods9101397
中图分类号
TS2 [食品工业];
学科分类号
0832 ;
摘要
The commercialization of porgies or seabreams of the family Sparidae has greatly increased in the last decade, and some valuable species have become subject to seafood substitution. DNA regions currently used for fish species identification in fresh and processed products belong to the mitochondrial (mt) genes cytochrome b (Cytb), cytochrome c oxidase I (COI), 16S and 12S. However, these markers amplify for fragments with lower divergence within and between some species, failing to provide informative barcodes. We adopted comparative mitogenomics, through the analysis of complete mtDNA sequences, as a compatible approach toward studying new barcoding markers. The intent is to develop a specific and rapid assay for the identification of the common pandora Pagellus erythrinus, a sparid species frequently subject to fraudulent replacement. The genetic diversity analysis (Hamming distance, p-genetic distance, gene-by-gene sequence variability) between 16 sparid mtDNA genomes highlighted the discriminating potential of a 291 bp NAD2 gene fragment. A pair of species-specific primers were successfully designed and tested by end-point and real-time PCR, achieving amplification only in P. erythrinus among several fish species. The use of the NAD2 barcoding marker provides a rapid presence/absence method for the identification of P. erythrinus.
引用
收藏
页数:15
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