Development of a rapid PCR protocol to detect Vibrio parahaemolyticus in clams

被引:18
|
作者
Federici, Sara [1 ]
Serrazanetti, Diana I. [2 ]
Guerzoni, M. Elisabetta [3 ]
Campana, Raffaella [1 ]
Ciandrini, Eleonora [1 ]
Baffone, Wally [1 ]
Gianotti, Andrea [2 ,3 ,4 ,5 ]
机构
[1] Univ Urbino Carlo Bo, Div Toxicol Hygien & Environm Sci, Dept Biomol Sci, Via S Chiara 27, I-61029 Urbino, Italy
[2] Univ Bologna, Interdept Ctr Ind Agri Food Res, Alma Mater Studiorum, Piazza Goidanich 60, I-47521 Cesena, Italy
[3] Univ Bologna, Dept Food Sci, Alma Mater Studiorum, Viale Fanin 46, I-40127 Bologna, Italy
[4] Univ Bologna, Dept Agr & Food Sci, Dipartimento Sci & Tecnol Agroalimentari DISTAL, Alma Mater Studiorum, Via Fanin 50, I-40127 Bologna, Italy
[5] Unita Org Cesena, Piazza Goidanich 60, Cesena, FC, Italy
来源
关键词
V; parahaemolyticus; Seafood; Detection method multiplex PCR; Real-time PCR; SHELLFISH; SEAFOOD; GENE; STRAINS; TDH; TRH; IDENTIFICATION; AMPLIFICATION; VULNIFICUS; OYSTERS;
D O I
10.1007/s13197-017-2986-9
中图分类号
TS2 [食品工业];
学科分类号
0832 ;
摘要
Vibrio parahaemolyticus is part of the natural microflora of estuarine and coastal marine waters and can be also present in seafood, especially shellfish and bivalve molluscs. In this study we compared the reference cultural method ISO 6887-3 with two molecular methods, multiplex PCR and real-time PCR, for the detection of two distinct genetic markers (tlh species-specific gene and tdh virulence gene) of V. parahaemolyticus in bivalve mollusc. The analyses were performed on clams inoculated with V. parahaemolyticus ATCC 43996 at T0 and after a 3 and 6 h of pre-enrichment in alkaline saline peptone water. Counts on agar plates were largely inaccurate, probably due to other Vibrio species grown on the TCBS selective agar. Multiplex PCR assays, performed using primers pairs for tdh and tlh genes, showed a detection limit of 10(4) CFU/g of shell stock within 6 h of pre-enrichment, respecting however the action level indicated by the National Seafood Sanitation Program guideline. Detection by tdh gene in real-time PCR reached the definitely highest sensitivity in shorter times, 10(1) CFU/g after 3 h of pre-enrichment, while the sensitivity for the tlh gene was not promising, detecting between 10(5) and 10(6) CFU/g after 6 h of pre-enrichment. Our findings provide a rapid routine method of detection of V. parahaemolyticus based on tdh gene by real-time PCR for commercial seafood analysis to identify the risk of gastrointestinal diseases.
引用
收藏
页码:749 / 759
页数:11
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