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Volume 3, Issue 2 (2014)                   J Police Med 2014, 3(2) | Back to browse issues page


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Zeinoddini M, Saeedinia A R, Sadeghi V. Rapid Detection of Vibrio Cholerae Using Hexaplex PCR Assay. J Police Med 2014; 3 (2)
URL: http://jpmed.ir/article-1-216-en.html
1- Assistant Professor, Department of Bioscience and Biotechnology, Malek Ashtar University of Technology, Tehran, Iran , zeinoddini@yahoo.com
2- PhD Student, Molecular Genetic, Department of Bioscience and Biotechnology, Malek Ashtar University of Technology, Tehran, Iran
3- MSc, Biotechnology, Department of Bioscience and Biotechnology, Malek Ashtar University of Technology, Tehran, Iran
English Extended Abstract:   (9573 Views)

Background: Vibrio cholerae is an important agent of diarrheal diseases in many parts of Asia and Africa. It is an enteric pathogen which produce a global pandemic of the disease. Rapid, sensitive and specific measurement of V. cholerae is an interest for many clinical laboratories. The aim of this study was to design and develop a hexaplex PCR assay for rapid detection of V. cholerae.

Materials and Methods: Six pair of primers were designed for specific amplification of the virulence and regulatory genes for Vibrio cholerae O1: cholera toxin enzymatic subunit A (ctxA) and B (ctxB), zonula occludens toxin (zot), accessory cholerae enterotoxin (ace), toxin- coregulated pilus (tcp) and outer membrane protein (ompW). Hexaplex PCR carried out using six primers and standard genes. Moreover, sensitivity and specificity of this method were determined.

Results: Hexaplex PCR showed the presence of the virulence and regulatory genes for Vibrio cholerae O1 in the standard sample. In addition, specificity was qualified and sensitivity determined 100 cfu/ml in this method.

Conclusion: Hexaplex PCR Assay could be used to design a kit for cholerae detection.

 

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Article Type: Original Research | Subject: Police Medicine Related Technologies
Received: 2014/06/2 | Accepted: 2014/09/7 | Published: 2014/10/12

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