Rapid and sensitive method for detection of Shiga-like toxin-producing Escherichia coli in ground beef using the polymerase chain reaction.

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Appl Environ Microbiol. 1992 December; 58(12): 3809-3815

Rapid and sensitive method for detection of Shiga-like toxin-producing Escherichia coli in ground beef using the polymerase chain reaction.

V P Gannon, R K King, J Y Kim and E J Thomas

Animal Diseases Research Institute, Agriculture Canada, Lethbridge, Alberta.

ABSTRACT

A rapid and sensitive method for detection of Shiga-like toxin(SLT)-producing Escherichia coli (SLT-EC) with the polymerasechain reaction (PCR) is described. Two pairs of oligonucleotideprimers homologous to SLTI and SLTII genes, respectively, wereused in multiplex PCR assays. The first pair generated a ca.600-bp PCR product with DNA from all SLTI-producing E. colitested but not from E. coli strains that produce SLTII or variantsof SLTII. The second pair generated a ca. 800-bp PCR productwith DNA from E. coli strains that produce SLTII or variantsof SLTII but not from SLTI-producing E. coli. When used in combination,the SLTI and SLTII oligonucleotide primers amplified DNA fromall of the SLT-EC tested. No PCR products were obtained withSLT primers with DNA from 28 E. coli strains that do not produceSLT or 44 strains of 28 other bacterial species. When groundbeef samples were inoculated with SLT-EC strains 319 (O157:H7;SLTI and SLTII), H30 (O26:H11; SLTI), and B2F1/3 (O91:H21; SLTIIvariants VT2ha and VT2hb) and cultured in modified Trypticasesoy broth for 6 h at 42 degrees C, an initial sample inoculumof as few as 1 CFU of these SLT-EC strains per g could be detectedin PCR assays with DNA extracted from the broth cultures.

Appl Environ Microbiol. 1992 December; 58(12): 3809-3815

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