Your search keyword '"Willshaw GA"' showing total 108 results

101. Expression of cloned plasmid regions encoding colonization factor antigen I (CFA/I) in Escherichia coli.

Author

Willshaw GA, Smith HR, McConnell MM, and Rowe B

Subjects

Bacterial Proteins genetics, Cloning, Molecular, DNA, Bacterial genetics, Escherichia coli immunology, Fimbriae, Bacterial immunology, Gene Expression Regulation, Genes, Bacterial, Antigens, Bacterial genetics, Escherichia coli genetics, Fimbriae Proteins, Plasmids

Abstract

Molecular cloning from a plasmid encoding colonization factor antigen I (CFA/I) and heat-stable enterotoxin isolated two regions, 1 and 2, that are required for the production of CFA/I fimbriae. The level of CFA/I synthesis measured by ELISA was similar in an Escherichia coli K12 strain carrying regions 1 and 2 cloned separately on compatible plasmid vectors to that in the same strain containing the parental plasmid. The structural gene for the CFA/I fimbrial subunit was within region 1. This region directed production in E. coli minicells of at least six independent polypeptides, of which the fimbrial subunit and at least three others appeared to be synthesized as precursor molecules that underwent processing. Cloned DNA containing CFA/I region 2 specified three polypeptides in minicells. Attempts to reduce the size of the cloned region 1 resulted in a derivative plasmid that carried the CFA/I structural gene but did not complement a region-2 recombinant plasmid to restore production of CFA/I fimbriae.

Published

1985

102. Properties of strains of Escherichia coli belonging to serogroup O157 with special reference to production of Vero cytotoxins VT1 and VT2.

Author

Scotland SM, Willshaw GA, Smith HR, and Rowe B

Subjects

Drug Resistance, Microbial, Escherichia coli isolation & purification, Humans, Neutralization Tests, Plasmids drug effects, Serotyping, Cytotoxins classification, Escherichia coli classification

Abstract

Fifty-four strains of Escherichia coli belonging to serogroup O157 were examined for the production of Vero cytotoxins VT1 and VT2, and for other properties such as plasmid content, resistance to antimicrobial agents and colicin production. Twenty-six strains from cases of diarrhoea, haemorrhagic colitis and haemolytic uraemic syndrome in humans produced VT. By serum neutralization tests and hybridization with DNA probes for VT1 or VT2, three classes were recognized which produced either VT1 alone or VT2 alone or both VT1 and VT2. These strains were of H type 7 or non-motile. The strains producing VT were sensitive to all the antimicrobial agents tested, and all carried at least one plasmid which had a molecular weight of c. 60 X 10(6). Seven strains of porcine origin and 21 strains of human origin did not produce VT or hybridize with either DNA probe. None of these strains was of H type 7. Of the 21 human VT- strains, 17 were of extra-intestinal origin and 18 were of H type 45. Twenty-three of the 28 VT-strains were resistant to at least one antimicrobial agent.

Published

1987

103. Heterogeneity of Escherichia coli phages encoding Vero cytotoxins: comparison of cloned sequences determining VT1 and VT2 and development of specific gene probes.

Author

Willshaw GA, Smith HR, Scotland SM, Field AM, and Rowe B

Subjects

Base Sequence, Cloning, Molecular, Coliphages ultrastructure, Cytotoxins genetics, DNA, Viral, Microscopy, Electron, Shiga Toxin 1, Bacterial Toxins genetics, Coliphages genetics

Abstract

Phages coding for production of Vero cytotoxins VT1 or VT2 in strains of Escherichia coli serotype O157.H7 or O157.H- were morphologically indistinguishable. Their genome size and restriction enzyme digests of the phage DNA were similar. These phages were clearly different in these respects from a VT1-encoding phage isolated from a strain of E. coli O26.H11 (H19). However the VT1 region cloned from the phage originating in the E. coli O157.H7 strain was identical to the VT1 region previously cloned from the phage carried by H19. Sequences encoding VT2 that were cloned from the phage in E. coli O157.H- have been mapped and the VT2 region identified by transposon insertion. The cloned regions coding for VT1 or VT2 production had no similarities in the presence of restriction enzyme sites over a distance of about 2 kb, and two VT1-specific probes spanning a region of about 1.4 kb did not hybridize under stringent conditions with cloned VT2 DNA. A 2 kb HincII fragment contained the VT2 genes but hybridized to VT1-encoding phages and recombinant plasmids via flanking phage DNA. A 0.85 kb AvaI-PstI fragment was a specific probe for VT2 sequences and did not hybridize under stringent conditions to phages or plasmid recombinants encoding VT1.

Published

1987

104. Mapping of a plasmid, coding for colonization, factor antigen I and heat-stable enterotoxin production, isolated from an enterotoxigenic strain of Escherichia coli.

Author

Smith HR, Willshaw GA, and Rowe B

Subjects

DNA Restriction Enzymes, DNA Transposable Elements, Deoxyribonuclease BamHI, Deoxyribonuclease EcoRI, Escherichia coli ultrastructure, Genetic Complementation Test, Hot Temperature, Mutation, Antigens, Bacterial genetics, Deoxyribonucleases, Type II Site-Specific, Enterotoxins genetics, Escherichia coli genetics, Fimbriae Proteins, Plasmids

Abstract

The non-autotransferring plasmid NTP113 codes for production of colonization factor antigen I and heat-stable enterotoxin, NTP113, which has a molecular weight of 58 X 10(6), was digested with BamHI, EcoRI, and HindIII and combinations of these restriction endonucleases, and the products of these digestions were analyzed by agarose gel electrophoresis. The results were used to construct a partial restriction map of NTP113. Transposons coding for resistance to ampicillin, kanamycin, and tetracycline were inserted into NTP113, and we obtained a series of deletion mutants, as determined by the loss of tetracycline or kanamycin resistance from strains carrying the insertion mutants. A number of plasmid mutants obtained by insertion or deletion did not code for colonization factor antigen I, but most of these mutants still coded for heat-stable enterotoxin production. The position of the inserted transposons and of the deletions were determined on the restriction map. Two regions of NTP113 were required for the expression of colonization factor antigen I, and the two sites were separated by a length of DNA corresponding to a molecular weight of about 25 X10(6).

Published

1982

105. Inhibition of Escherichia coli isoleucine biosynthesis by isoleucine tetrazole.

Author

Willshaw GA and Tristram H

Subjects

2-Isopropylmalate Synthase metabolism, Acetolactate Synthase metabolism, Depression, Chemical, Drug Resistance, Microbial, Escherichia coli growth & development, Homoserine pharmacology, Isoleucine analogs & derivatives, Isoleucine pharmacology, Isoleucine-tRNA Ligase metabolism, Membrane Transport Proteins metabolism, Methionine pharmacology, Mutation, Peptides pharmacology, Tetrazoles antagonists & inhibitors, Threonine pharmacology, Threonine Dehydratase metabolism, Valine pharmacology, Azoles pharmacology, Escherichia coli metabolism, Isoleucine biosynthesis, Tetrazoles pharmacology

Abstract

Growth of a derivative of Escherichia coli K-10 was strongly inhibited by 2 times 10(-4) M L-5(1-amino-2-methylbutyl)-tetrazole (isoleucine tetrazole). Growth inhibition was reversed by isoleucine, threonine, glycyl-L-isoleucine, or glycyl-L-threonine, and, in a valine-resistant mutant, by L-valine. Partial reversal of growth inhibiton was effected by L-leucine, L-methionine, or L-homoserine. The tetrazole inhibited the activity of the biosynthetic threonine deaminase (EC 4.2.1.16 L-threonine hydrolyase [deaminating]), the inhibition being relieved by L-valine. The tetrazole also inhibited isoleucyl-transfer ribonucleic acid (tRNA) synthetase (EC 6.1.1.5 L-isoleucine: tRNA ligase [adenosine monophosphate]), but was without effect on the activities of alpha-isopropylmalate synthetase or acetohydroxy acid synthetase. One class of isoleucine tetrazole-resistant mutants produced biosynthetic threonine deaminases which were no longer subject to feedback inhibition by either isoleucine or the tetrazole.

Published

1975

106. Vero cytotoxin production and presence of VT genes in Escherichia coli strains of animal origin.

Author

Smith HR, Scotland SM, Willshaw GA, Wray C, McLaren IM, Cheasty T, and Rowe B

Subjects

Animals, Bacterial Toxins genetics, Cattle, DNA, Bacterial, Escherichia coli metabolism, Nucleic Acid Hybridization, Shiga Toxin 1, Swine, Bacterial Toxins biosynthesis, Escherichia coli genetics, Genes, Bacterial

Abstract

Vero cytotoxin (VT) production has been studied in 34 Escherichia coli strains isolated from animals with enteric diseases. The strains were tested by DNA hybridization with probes for VT1 and VT2 sequences and also in toxin neutralization experiments with specific antisera. Twenty bovine strains, belonging to nine different O serogroups, produced VT1 or VT2 but not both toxins. In contrast, all 14 porcine strains of four different O serogroups produced VT2 only. Six of these porcine strains, belonging to serogroups O138, O139 and O141, were isolated from cases of oedema disease. In general, the porcine isolates produced toxin at a lower level than the bovine strains.

Published

1988

107. The nucleotide sequence of the first two genes of the CFA/I fimbrial operon of human enterotoxigenic Escherichia coli.

Author

Hamers AM, Pel HJ, Willshaw GA, Kusters JG, van der Zeijst BA, and Gaastra W

Subjects

Amino Acid Sequence, Base Sequence, Blotting, Southern, Codon, Computer Simulation, DNA Transposable Elements, DNA, Bacterial genetics, Humans, Molecular Sequence Data, Nucleic Acid Conformation, Plasmids, Promoter Regions, Genetic, Regulatory Sequences, Nucleic Acid, Restriction Mapping, Ribosomes metabolism, Sequence Homology, Nucleic Acid, Transformation, Genetic, Antigens, Bacterial genetics, Escherichia coli genetics, Fimbriae Proteins, Fimbriae, Bacterial immunology, Genes, Bacterial, Operon

Abstract

An oligonucleotide probe, derived from the N-terminal amino acid sequence of the CFA/I fimbrial subunit protein, was used to identify the gene encoding this protein within a cloned DNA fragment encoding CFA/I fimbriae. The gene (cfa b) was found and sequenced. Flanking it upstream was a gene (cfa a) encoding a protein of 206 amino acids and downstream a gene (cfa c) probably encoding an 85 kDa protein was found. This genetic organisation of the CFA/I operon differs from that of other fimbrial operons in Escherichia coli. All three proteins have signal peptides. The nucleotide sequence was analysed for homology with other sequences, secondary structure, ribosomal binding sites and possible promoter sequences. A region of dyad symmetry probably involved in the regulation of translation of the cfa c gene was found at the 5' end of this gene. A region of dyad symmetry was also observed within the cfa b gene. In front of the CFA/I operon part of insertion sequence IS2 was found. This IS2 sequence was found in a number of CFA/I plasmids, obtained from strains isolated from various geographic locations. The insertion of the IS2 element in the CFA/I operon therefore probably happened rather early during evolution of CFA/I producing Escherichia coli strains.

Published

1989

108. Adhesion to cells in culture and plasmid profiles of enteropathogenic Escherichia coli isolated from outbreaks and sporadic cases of infant diarrhoea.

Author

Scotland SM, Willshaw GA, Smith HR, Gross RJ, and Rowe B

Subjects

Cell Line, Diarrhea, Infantile epidemiology, Escherichia coli classification, Escherichia coli genetics, Escherichia coli isolation & purification, Escherichia coli Infections epidemiology, Humans, Infant, Infant, Newborn, Nucleic Acid Hybridization, United Kingdom, Bacterial Adhesion, Diarrhea, Infantile microbiology, Disease Outbreaks, Escherichia coli physiology, Escherichia coli Infections microbiology, Plasmids

Abstract

Enteropathogenic strains of Escherichia coli (EPEC) that caused 10 outbreaks of infant diarrhoea in the U.K. between 1968 and 1986 were studied. All gave localised adherence (LA) to HEp-2 cells, HeLa cells and Intestine 407 cells in culture. All hybridised with the EPEC adherence factor (EAF) probe. The hybridising sequences were carried on plasmids ranging in size from 26 to 76 MDa. EPEC from sporadic cases of infant diarrhoea occurring between 1979 and 1986 that belonged to the same serotypes as the outbreak strains were also studied. All strains of serotypes O111ab.H2, O114.H2, O119.H6, O127.H6 and O142.H6 gave LA and were EAF-positive. In other serotypes, non-adhering strains or strains giving diffuse adherence were found also. In addition, strains of serotype O128.H2 which gave LA but did not hybridise with the EAF probe were identified. The strains isolated from sporadic cases of diarrhoea in the U.K. were similar, with respect to adhesion and hybridisation, to those isolated from sporadic cases of diarrhoea in developing countries.

Published

1989