AI Article Synopsis

  • The study compared three methods (agar plate cultivation, immunofluorescence antibody technique, and nested PCR) for detecting the pathogen Flavobacterium psychrophilum in farmed salmonid fish environments.
  • Nested PCR was found to be the most sensitive method, detecting the pathogen at much lower concentrations than the other methods (3 CFU/ml for PCR vs. 32 CFU/ml for agar and 410 cells/ml for IFAT).
  • IFAT and nested PCR were more effective and rapid for detection in water samples from fish farms, while agar plate cultivation was less successful in isolating the pathogen.

Article Abstract

Rainbow trout fry syndrome and cold-water disease are serious diseases in farmed salmonid fish. In the present study, three methods were compared, for the detection of the causative pathogen, Flavobacterium psychrophilum in water. The methods included traditional agar plate cultivation on tryptone yeast extract salts (TYES) agar, immunofluorescence antibody technique (IFAT) and nested PCR. The three methods were subsequently used for the detection of F. psychrophilum from fish farm environments. The nested PCR was the most sensitive method used for a detection of F. psychrophilum. As low as 3 CFU estimated by agar plate cultivation or 41 cells estimated by IFAT of F. psychrophilum per ml of non-sterile well water were needed for a detection using the nested PCR method. The obtained detection limits for the agar plate cultivation and the IFAT was 32 CFU/ml and 410 cells/ml, respectively. Using IFAT and nested PCR F. psychrophilum was detected most frequently in water samples from fish farms, but the pathogen was isolated from only a few samples using agar plate cultivation. In the present study IFAT and nested PCR proved to be rapid, specific and sensitive methods compared to traditional agar plate cultivation for the detection of F. psychrophilum from environmental samples. It is suggested that IFAT and nested PCR provide effective tools for the examination of F. psychrophilum in the environment.

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Source
http://dx.doi.org/10.1078/0723-2020-00105DOI Listing

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