Pregled bibliografske jedinice broj: 111574
Yersinia spp. direct detection in food by molecular methods.
Yersinia spp. direct detection in food by molecular methods. // ? Quality and risk assessment of agricultural food in the Mediterranean area"
Foggia, Italija, 2002. (predavanje, međunarodna recenzija, sažetak, ostalo)
CROSBI ID: 111574 Za ispravke kontaktirajte CROSBI podršku putem web obrasca
Naslov
Yersinia spp. direct detection in food by molecular methods.
(Direktno odredjivanje Yersina spp. u hrani pomocu molekularnih metoda)
Autori
Cocolin, Luca ; Orlić, Sandi ; Iacumin, Lucilla ; Manzano, Marisa ; Comi, Giuseppe
Vrsta, podvrsta i kategorija rada
Sažeci sa skupova, sažetak, ostalo
Skup
? Quality and risk assessment of agricultural food in the Mediterranean area"
Mjesto i datum
Foggia, Italija, 24.09.2002. - 27.09.2002
Vrsta sudjelovanja
Predavanje
Vrsta recenzije
Međunarodna recenzija
Ključne riječi
Yersinia spp.; food; detection
Sažetak
Yersinia is well established as a foodborne pathogen of human concern and is most frequently associated with raw and cooked meat products. The genus Yersinia comprises 11 species, of which Y. pestis, Y. pseudotubercolosis and Y. enterocolitica posses the potential to be pathogenic in humans and animals. The pathogenicity of these three strains is controlled by the common 64- to 75-Kb virulence plasmid. Strains of Y. enterocolitica non- plasmid-bearing are not virulent. Those isolates formerly called Y. enterocolitica-like isolates were reclassified and assigned to eight different species (Y. frederiksenii, Y. intermedia, Y. kristensenii, Y. mollareti, Y. bercoveri, Y. aldovae, Y. rhodei and Y. ruckeri). Traditional methods employ the use of prolonged enrichments at refrigeration temperatures to take advantage of phychrotrophic nature of Yersinia and to suppress the growth of background flora. Due to the extended time period needed for this type of method, efforts have been made to devise selective enrichment techniques employing shorter incubation times and higher temperatures, thus making more practical for routine use. With the development of new molecular techniques more powerful protocols have became available to improve the quality of the food microbiological analysis. The recent developed techniques for amplifying specific DNA sequences in vitro allow the detection of infinitesimally small amounts of target DNA in various environment and food specimens. In this study the Yersinia spp., more frequent isolated from food, were considered to optimize a PCR-Denaturing Gradient Gel Electrophoresis (DGGE) to allow their direct detection in food samples. A couple of primers targeting the rpoB gene were used to produce a 350 bp PCR amplicon that was subsequently subjected to DGGE analysis. The protocol was optimized by using strains from international collections, then applied for the identification of Yersinia spp. isolated traditionally from food samples and at last for the direct identification of yersiniae. The application of the PCR-DGGE protocol allowed to obtain species-specific patterns for the species used in the study, highlighting the possibility to apply the method for a direct detection and identification of Yersinia spp. in food samples.
Izvorni jezik
Engleski
