Comparison of Western immunoblots and gene detection assays for identification of potentially enterotoxigenic isolates of Clostridium perfringens.

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J Clin Microbiol. 1994 October; 32(10): 2533-2539

Comparison of Western immunoblots and gene detection assays for identification of potentially enterotoxigenic isolates of Clostridium perfringens.

J F Kokai-Kun, J G Songer, J R Czeczulin, F Chen and B A McClane

Department of Molecular Genetics and Biochemistry, University of Pittsburgh School of Medicine, Pennsylvania 15261-2072.

ABSTRACT

Clostridium perfringens enterotoxin (CPE) is an important sporulation-associatedvirulence factor in several illnesses of humans and domesticanimals, including C. perfringens type A food poisoning. Therefore,the ability to determine the enterotoxigenicity of food or fecalC. perfringens isolates with simple, rapid assays should behelpful for epidemiologic investigations. In this study, Westernimmunoblotting (to detect CPE production in vitro) was comparedwith PCR assays and digoxigenin-labeled probe assays (to detectall or part of the cpe gene) as a method for determining theenterotoxigenicity of C. perfringens isolates. The cpe detectionassays yielded reliable results with DNA purified from vegetativeC. perfringens cultures, while Western immunoblots requiredin vitro sporulation of C. perfringens isolates to detect CPEproduction. Several cpe-positive C. perfringens isolates fromdiarrheic animals did not sporulate in vitro under commonlyused sporulation-inducing conditions and consequently testedCPE negative. This result indicates that cpe gene detectionand serologic CPE assays do not necessarily yield similar conclusionsabout the enterotoxigenicity of a C. perfringens isolate. Untilfurther studies resolve whether these cpe-positive isolateswhich do not sporulate in vitro can or cannot sporulate andproduce CPE in vivo, it may be preferable to use cpe detectionassays for evaluating C. perfringens isolate enterotoxigenicityand thereby avoid potential false-negative conclusions whichmay occur with serologic assays.

J Clin Microbiol. 1994 October; 32(10): 2533-2539

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