Korean Journal of Veterinary Research (대한수의학회지)

The Korean Society of Veterinary Science (대한수의학회)
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Rapid diagnosis of experimental listeriosis in mice by polymerase chain reaction

중합효소연쇄반응을 이용한 실험적 리스테리아 감염증의 신속진단

  • Kang, Ho-jo (College of Veterinary Medicine Gyeonsang National University) ;
  • Lee, Seong-mi (College of Veterinary Medicine Gyeonsang National University) ;
  • Suk, Ju-myoung (Institute of Animal Medicine, Gyeongsang Natinal University) ;
  • Lee, Deog-kyu (Masan Junior College) ;
  • Son, Won-geun (Health Canada, Animal Disease Research Institute, Canadian Food Inspection Agency)
  • 강호조 (경상대학교 수의과대학) ;
  • 이성미 (경상대학교 수의과대학) ;
  • 석주명 (경상대학교 동물의학연구소) ;
  • 이덕규 (마산전문대학 방사선과) ;
  • 손원근 (캐나다 식품검사국)
  • Received : 1998.04.14
  • Published : 1998.09.25
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Abstract

The polymerase chain reaction(PCR) assay was used for rapid diagnosis from blood and organ samples experimentally infected with Listeria monocytogenes. This method used a pair of primers based on a unique region in the 16S rRNA sequence of L monocytogenes. Procedure A was based on dilution of the blood sample followed by lysis of bacterial cell and direct analysis of the lysate with PCR. In artificially infected blood samples with L monocytogenes, it was possible to detect fewer than 40 cells per ml of blood. However, L monocytogenes was detected low rates on infected organs by the direct PCR. In procedure B, enrichment cultivation was used to increase numbers of bacteria before lysis and PCR. L monocytogenes was detected from 23 samples of 24 liver and spleen, respectively, and 18 samples of 24 blood were found to be positive by PCR on a subset of 72 organ samples, whereas L monocytogenes were detected on 63 organ samples in classical culture technique. It was required to analyze including enrichment steps were 6h and 18h on the procedure A and B, respectively.

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