A search for cholera toxin (CT), toxin coregulated pilus (TCP), the regulatory element ToxR and other virulence factors in non-O1/non-O139Vibrio cholerae

• Published in: Microbial pathogenesis Vol. 22; no. 4; pp. 199 - 208
• Main Authors: Ghosh, Chandradipa, Nandy, Ranjan K., Dasgupta, Sujoy K., Balakrish Nair, G., Hall, Robert H., Ghose, Asoke C.
• Format: Journal Article
• Language: English
• Published: Elsevier Ltd 01.04.1997
• Subjects: cholera toxin; Non-O1V. cholerae; toxin coregulated pilus; virulence factors; Non-O1V. cholerae; toxin coregulated pilus; cholera toxin; virulence factors
• ISSN: 0882-4010; 1096-1208
• DOI: 10.1006/mpat.1996.0105

Twenty-four selected non-O1/non-O139Vibrio choleraestrains were examined for the presence of virulence associated genes likectxA,tcpA,toxRand the repetitive sequence (RS element). Seventeen of these were isolated from diarrhoeal stool samples while the remaining seven were of local environmental origin. Nine and four respectively of these strains were positive forctxAandtcpAby Multiplex PCR analysis. The majority (16 out of 18 tested) of the strains (including the fourtcpA+ strains) containedtoxRsequences as determined by another PCR assay. The presence of RS element was demonstrable inctxA+strains only. Interestingly, three of these non-O1/non-O139 strains were shown to contain all the three virulence associated genes (ctxA,tcpAandtoxR) as well as the RS element. Two of these belonged to serogroups 037 (V2) and 064 (CG15) while the third one (V315-1) was untypable. These three strains also produced cholera toxin, expressed toxin coregulated pilus (TCP) and/or TcpA related antigens when grown under appropriate culture conditions. Southern hybridization analysis of their chromosomal DNA fragments using DNA probes representingctxA, zot, aceand RS element revealed that the strains V2 and CG15 contained, at least, two complete copies of the CTX genetic element, while the strain V315-1 had three or more copies of the same. Presence of the RS element in these strains led to tandem duplication of the CTX genetic element in the chromosome of V2 and V315-1, but not in CG15 where the copies were likely to be present at different loci. These results also indicate the presence of additional copies of incomplete ‘core region’ withzotandacegenes, but notctxA, in strains V2 and CG15. The significance of these results in terms of the pathogenic and epidemic potential ofV. choleraestrains is discussed.