Cloning and expression of the genes specifying Shiga-like toxin production in Escherichia coli H19

Huang, Annie; Grandis, S De; Friesen, James D.; Karmali, M A; Petric, Martin; Congi, R V; Brunton, James

doi:10.1128/jb.166.2.375-379.1986

Cited by 84 publications

(63 citation statements)

References 24 publications

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“…VT genes have been cloned in E. coli strain K12 from phages originating in strains of serogroups 026 and 0157 (Newland et al, 1985;Willshaw et al, 1985Huang et al, 1986). The VT1 region cloned from a strain of serogroup 0157 was very similar to the VT1 sequences cloned from strain H19 in the distribution of sites for several restriction enzymes.…”

Section: Genetics Of Vt Productionmentioning

confidence: 99%

Vero cytotoxin-producing strains of Escherichia coli

Smith

Scotland

1988

Journal of Medical Microbiology

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Section: Genetics Of Vt Productionmentioning

confidence: 99%

Vero cytotoxin-producing strains of Escherichia coli

Smith

Scotland

1988

Journal of Medical Microbiology

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“…Goat antimouse and antirabbit IgG horseradish peroxidase conjugates were from Sigma. Verotoxin-1 was purified from the recombinant strain pJLB28 [24] as described [25]. Toxin was radioiodinated using iodobeads (Pierce) [13].…”

Section: Methodsmentioning

confidence: 99%

Lipid modulation of glycolipid receptor function

Boyd

Magnusson

Zhiuyan

et al. 1994

European Journal of Biochemistry

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Verotoxins bind to glycosphingolipids containing terminal Gal(a1-4)Gal residues. Globotriaosylceramide is the most effective receptor for verotoxin-1 in vitro and is the functional plasma-membrane receptor which mediates cytopathology for most sensitive cells. Binding of verotoxin-1 to a series of galabiose-containing or globotriaose-containing synthetic glycolipids with monoalkylsulfides and bisalkylsulfides or sulfones as the lipid moiety, have been studied for toxin binding by TLC overlay and in solid phase in the presence of auxiliary lipids. The results demonstrate that for an identical carbohydrate, binding is dramatically altered according to the nature of the lipid moiety. The close proximity of the galabiose sequence and the hydrophobic species also compromised recognition.The lipid environment is also a major determinant of receptor function, since species that were effective, even preferred toxin receptors as monitored by TLC overlay, were not necessarily recognized in the presence of auxiliary lipids. Certain glycolipids, which were not recognized by TLC overlay, were nevertheless found to be effective receptors in an auxiliary lipid matrix.These results demonstrate the crucial role of the lipid moiety in verotoxidglycolipid recognition and are discussed in relation to toxin pathogenesis and glycolipid receptor function.The Escherichia coli-derived verotoxin is a subunit toxin comprising five receptor-binding B subunits and one noncovalently associated A subunit, which is responsible for intracellular inhibition of protein synthesis [I, 21. Several verotoxin isotypes have been described. Verotoxin-1 is nearly identical to Shiga toxin from Shigella dystenteriae and verotoxins are, therefore, also referred to as Shiga-like toxins [31. The nomenclature within this toxin family has been confusing but a consensus has been proposed [4].Infection with verotoxin-producing E. coli is strongly associated with hemorrhagic colitis [S] and the hemolytic uremic syndrome [6] in humans. It is believed that the toxin targets endothelial cells within the gastrointestinal vasculature and renal glomerulus. The glycolipid globotriaosylceramide [GbOse, ; Gal(al-4)Gal(pl-4)Glc pl-*ceramide] is recognized by the human verotoxins (verotoxin-1, verotoxin-2 and verotoxin-2c) in various in vitro binding assays [7] and has been shown to mediate the pathology in sensitive cells in vitro [8, 91. GbOse, is a major component of the Abbreviations. GaOsez or galabiosyl ceramide, Gal(a1-4)Gal ceramide; GbOse, or globotriaosyl ceramide, Gal(al-4)GalVl-4)Glc ceramide ; GbOse, or globotetraosyl ceramide, GalNacVl -3)Gal(nl-4)Ga1(~1-4)Glc ceramide. glycolipid fraction of the human kidney cortex [lo], particularly the glomerular endothelial cells [ 1 11 and glycolipid binding may therefore determine the cytopathology in vivo. The pig edema toxin (verotoxin-2e) preferentially recognises GbOse, [GalNac(pl-3)Gal(al-4)Gal(pl-4)GlcCer] in addition to GbOse, and thus is the only member of the toxin family to recognize an internally placed galabio...

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“…The latter scenario is predominantly found in bacterial species and accounts for lysogenic conversions, phenomena in which phenotypes of the microbial host including pathogenicity, growth performance and production of virulence factors and toxins can be significantly affected by expression of prophage encoded genes. Prominent examples for phage-dependent toxin expression and disease formation include exotoxin-associated scarlet fever by Streptocoocus pyogenes (Johnson et al, 1986;Broudy et al, 2001), dysentery causing Shiga toxins Stx1 and Stx2 from Shigella dysenteriae (Newland et al, 1985;Willshaw et al, 1985;Huang, et al, 1986), phage CTXφ encoded cholera toxin from Vibrio cholera (Waldor & Mekalanos, 1996;Faruque & Nair, 2002) and diphtheria toxin encoded on a beta prophage from lysogens of Corynebacterium diphtheriae (Holmes & Barksdale, 1969;Bishai & Murphy 1988). Together 334 with tRNase ribotoxins and anticodon nucleases from prokaryal and eukaryal microbes that have been shown to be encoded by transposable elements as well as circular and nonconventional linear DNA plasmids (Tokunaga et al, 1990;Kaufmann, 2000;Schaffrath & Meinhardt, 2005;Schaffrath et al, 1999), all of these genetic constellations implicate scenarios in which killer phenotypes have been evolved and spread by way of viral DNA transduction pathways or other forms of horizontal gene transfer.…”

Section: Introductionmentioning

confidence: 99%