1988
DOI: 10.1007/bf01941182
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Development of DNA probes for cytotoxin and enterotoxin genes in enteric bacteria

Abstract: DNA probes to identify the genes encoding toxins in enteric bacteria have been developed. Use of these probes reduces the number of animals required for toxicity testing, as suspect bacteria can be directly tested for the presence of toxin. We have augmented the gene probes available by developing probes against the Escherichia coli enterotoxin LTII and shiga toxin from Shigella dysenteriae 1. The LTII gene from E. coli 357900 was identified and characterised and a suitable internal probe was obtained. The LTI… Show more

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Cited by 5 publications
(3 citation statements)
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“…In conclusion, the 800 bp ClaI-EcoRI fragment, encoding the stn gene can be utilized as a probe in the identification of bacterial strains that encode similar enterotoxins, and study their 91 phylogenetic relationships [18,19]. Overexpression of STN in the T7 RNA polymerase/promoter system should help in understanding the native structure of the protein and study of its mode of action.…”
Section: Properties Of the Stn Gene Productmentioning
confidence: 99%
“…In conclusion, the 800 bp ClaI-EcoRI fragment, encoding the stn gene can be utilized as a probe in the identification of bacterial strains that encode similar enterotoxins, and study their 91 phylogenetic relationships [18,19]. Overexpression of STN in the T7 RNA polymerase/promoter system should help in understanding the native structure of the protein and study of its mode of action.…”
Section: Properties Of the Stn Gene Productmentioning
confidence: 99%
“…One SLT-II isolate also produced LT-II, as did 7 of 30 isolates subsequently found to have lost SLT activity. Only three of these eight isolates were LT-IIa probe positive, while all were positive with a probe derived from the LT-II toxin locus from isolate 357900 [53], which we have here determined to encode LT-IIc1. These two probes have a 749 bp region in common that encodes parts of the A and B genes, 343 bp of which are 96% identical (A1 gene) and 406 bp of the A2 and B genes that shows only 59% identity.…”
Section: Discussionmentioning
confidence: 79%
“…The molecular mass markers are indicated on the left, and from top to bottom they are 97. 4 tac promoter with the synthetic modified 3-lactamase or the aerobactin not clear but it seems likely that the S. typhimunium aroA strains have additional mutations which cause the defect in the export process. These strains are not, however, defective in the transport of other outer membrane proteins normally found in wild-type S. typhimurium, and hence, it seems unlikely that any of the "chaperone" proteins of the Sec-mediated protein translocation pathway (for reviews on the Sec pathway, see reference 1) are mutated.…”
Section: Discussionmentioning
confidence: 99%