Molecular typing of toxigenic Clostridum perfringens isolated from sheep in Iran
2011
Jabbari, A.R., Department of Anaerobic bacterial vaccine research & production, Razi vaccine and serum research institute, Karaj, Iran | Afshari Far, S., Department of Biotechnology, Razi vaccine and serum research institute, Karaj, Iran | Esmaelizad, M., Faculty of Basic Sciences, Payame Noor University, Tehran, Iran | Pilehchian Langroudi, R., Department of Anaerobic bacterial vaccine research & production, Razi vaccine and serum research institute, Karaj, Iran | Moosawi shooshtari, M., Department of Anaerobic bacterial vaccine research & production, Razi vaccine and serum research institute, Karaj, Iran | Abdolmohammadi Khiav, L., Department of Anaerobic bacterial vaccine research & production, Razi vaccine and serum research institute, Karaj, Iran
In this research a molecular method based on polymerase chain reaction for typing of Clostridium perfringens was developed and toxin genotypes of 64 isolates from sheep and goats in Iran were determined. The PCR assays were developed for detection of alpha ( cpa ) , beta ( cpb ) and epsilon ( etx ) toxin genes, allowing classification of the isolates into genotypes A B, C and D. The field isolates were assigned to genotypes A ( n=9, 14.07 %) , B ( n=20, 31.25% ) , C ( n=17, 26.56%) and D ( n=18, 28.12% ) . In this PCR system the fragments of 900, 611 and 402 bp were amplified using specific primers for alpha, beta and epsilon toxins, respectively. The fragments were confirmed by sequencing and blasting in GenBank. The sequence alignment of the fragments showed more than 98% similarity with other related published sequences from other sources. Our results suggest that PCR genotyping is an acceptable tool for in vitro typing of C. perfringens
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