Comparison of DNA fingerprinting methods for use in investigation of type E botulism outbreaks in the Canadian arctic

Pulsed-field gel electrophoresis (PFGE), randomly amplified polymorphic DNA (RAPD) analysis, and automated ribotyping were compared for epidemiological typing of Clostridium botulinum type El using clinical and food isolates associated with four botulism outbreaks occurring in the Canadian Arctic. All type E strains previously untypeable by PFGE, even with the use of a formaldehyde fixation step, could be typed by the addition of 50 mu M thiourea to the electrophoresis running buffer. Digestion with SmaI or Xhol followed by PFGE was used to link food and clinical isolates from four different type E botulism outbreaks and differentiate them from among 39 group II strains. Strain differentiation was unsuccessful with the automated ribotyping system, producing a single characteristic EcoRI fingerprint common to all group II strains. RAPD analysis of C. botulinum group II strains was not consistently reproducible with primer OPJ-6 or OPJ-13. apparently discriminating between epidemiologically related strains. A modified PFGE protocol was judged to he the most useful method for typing epidemiologically related C. botulinum type E, strains, based on its ability to type all strains reproducibly and with an adequate level of discrimination.