Application of 5'-Nuclease PCR for Quantitative Detection of Listeria monocytogenes in Pure Cultures, Water, Skim Milk, and Unpasteurized Whole Milk

doi:10.1128/AEM.66.10.4266-4271.2000

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Applied and Environmental Microbiology, October 2000, p. 4266-4271, Vol. 66, No. 10
0099-2240/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Application of 5'-Nuclease PCR for Quantitative Detection of Listeria monocytogenes in Pure Cultures, Water, Skim Milk, and Unpasteurized Whole Milk

Hege Karin Nogva,^* Knut Rudi, Kristine Naterstad, Askild Holck, and Dag Lillehaug

MATFORSK, Norwegian Food Research Institute, N-1430 Ås, Norway

Received 13 March 2000/Accepted 27 June 2000

PCR techniques have significantly improved the detection and identification of bacterial pathogens. Countless adaptationsand applications have been described, including quantitative PCRand the latest innovation, real-time PCR. In real-time PCR, e.g.,the 5'-nuclease chemistry renders the automated and direct detectionand quantification of PCR products possible (P. M. Holland etal., Proc. Natl. Acad. Sci. USA 88:7276-7280, 1991). We presentan assay for the quantitative detection of Listeria monocytogenesbased on the 5'-nuclease PCR using a 113-bp amplicon from thelisteriolysin O gene (hlyA) as the target. The assay was positivefor all isolates of L. monocytogenes tested (65 isolates includingthe type strain) and negative for all other Listeria strains (16isolates from five species tested) and several other bacteria(18 species tested). The application of 5'-nuclease PCR in diagnosticsrequires a quantitative sample preparation step. Several magneticbead-based strategies were evaluated, since these systems aresimple and relatively easy to automate. The combination of nonspecificbinding of bacteria to paramagnetic beads, with subsequent DNApurification by use of the same beads, gave the most satisfactoryresult. The detection limit was approximately 6 to 60 CFU, quantificationwas linear over at least 7 log units, and the method could becompleted within 3 h. In conclusion, a complete quantitative methodfor L. monocytogenes in water and in skimmed and raw milk wasdeveloped.

^* Corresponding author. Mailing address: MATFORSK, Osloveien 1, N-1430 Ås, Norway. Phone: 47-64-97-01-00. Fax: 47-64-97-03-33.E-mail: hege.nogva{at}matforsk.no.

Present address: Norwegian Food Control Authority, N-0034 Oslo,Norway.

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