A polymerase chain reaction assay was developed for detection of the Vibrio cholerae heat-stable enterotoxin gene (sto). The assay is based on two oligonucleotide primers suitable for amplification of the entire sto open reading frame. Reaction conditions were defined to obtain optimal results in terms of specificity and sensitivity. Under these conditions the assay was highly sensitive and enabled good results to be obtained using as a template crude DNA preparations from single bacterial colonies. A rapid protocol for direct sequence analysis of the amplification product which may be used in combination with the PCR assay to confirm the product identity and analyse sequence polymorphisms within the sto gene, was also developed. Twenty-two V. cholerae non O-1 isolates from sporadic cases of V. cholerae non-O1- associated gastroenteritis from Cuba were analysed by this PCR assay. Four strains (18.2%) were found to carry the sto gene. The prevalence of V. cholerae non-O1 strains carrying the sto gene among clinical isolates is higher than that reported for other geographical areas except in the case of epidemics. © 1994 Academic Press limited.
Guglielmetti, P., Bravo, L., Zanchi, A., Montè, R., Lombardi, G., Rossolini, G.M. (1994). Detection of the Vibrio cholerae heat-stable enterotoxin gene by polymerase chain reaction. MOLECULAR AND CELLULAR PROBES, 8(1), 39-44 [10.1006/mcpr.1994.1005].
Detection of the Vibrio cholerae heat-stable enterotoxin gene by polymerase chain reaction
Rossolini G. M.
1994-01-01
Abstract
A polymerase chain reaction assay was developed for detection of the Vibrio cholerae heat-stable enterotoxin gene (sto). The assay is based on two oligonucleotide primers suitable for amplification of the entire sto open reading frame. Reaction conditions were defined to obtain optimal results in terms of specificity and sensitivity. Under these conditions the assay was highly sensitive and enabled good results to be obtained using as a template crude DNA preparations from single bacterial colonies. A rapid protocol for direct sequence analysis of the amplification product which may be used in combination with the PCR assay to confirm the product identity and analyse sequence polymorphisms within the sto gene, was also developed. Twenty-two V. cholerae non O-1 isolates from sporadic cases of V. cholerae non-O1- associated gastroenteritis from Cuba were analysed by this PCR assay. Four strains (18.2%) were found to carry the sto gene. The prevalence of V. cholerae non-O1 strains carrying the sto gene among clinical isolates is higher than that reported for other geographical areas except in the case of epidemics. © 1994 Academic Press limited.I documenti in IRIS sono protetti da copyright e tutti i diritti sono riservati, salvo diversa indicazione.
https://hdl.handle.net/11365/29035
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