Chemical synthesis of an octadecapeptide with the biological and immunological properties of human heat-stable Escherichia coli enterotoxin

Houghten, Richard A.; Ostresh, John M.; Klipstein, Frederick A.

doi:10.1111/j.1432-1033.1984.tb08535.x

Cited by 35 publications

(44 citation statements)

References 25 publications

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“…With the relatively stable conotoxin GI, partial reduction by NaBH, in the presence of iodoacetic acid gave unambiguous results (Gray et al, 1984), although some exchange was detected. On the other hand, alkylation of partially oxidized enterotoxin led to incorrect assignments (Houghten et al, 1984). The present work describes a way to circumvent the exchange problem, opening a new route to disulfide assignment.…”

Section: Discussionmentioning

confidence: 92%

Disulfide structures of highly bridged peptides: A new strategy for analysis

1993

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A new approach is described for analyzing disulfide linkage patterns in peptides containing tightly clustered cystines. Such peptides are very difficult to analyze with traditional strategies, which require that the peptide Chain be split between close or adjacent Cys residues. The water-soluble tris-(2-~arboxyethyl)-phosphine (TCEP) reduced disulfides at pH 3, and partially reduced peptides were purified by high performance liquid chromatography with minimal thiol-disulfide exchange. Alkylation of free thiols, followed by sequencer analysis, provided explicit assignment of disulfides that had been reduced. Thiol-disulfide exchange occurred during alkylation of some peptides, but correct deductions were still possible. Alkylation competed best with exchange when peptide solution was added with rapid mixing to 2.2 M iodoacetamide. Variants were developed in which up to three alkylating agents were used to label different pairs of thiols, allowing a full assignment in one sequencer analysis. Model peptides used included insulin (three bridges, intra-and interchain disulfides; -Cys.Cys-pair), endothelin and apamin (two disulfides; -Cys.x.Cys-pair), conotoxin GI and isomers (two disulfides; -Cys.Cys-pair), and bacterial enterotoxin (three bridges within 13 residues; two -Cys.Cys-pairs). With insulin, all intermediates in the reduction pathway were identified; with conotoxin GI, analysis was carried out successfully for all three disulfide isomers. In addition to these known structures, the method has been applied successfully to the analysis of several previously unsolved structures of similar complexity. Rates of reduction of disulfide bonds varied widely, but most peptides did not show a strongly preferred route for reduction.

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Section: Discussionmentioning

confidence: 92%

Disulfide structures of highly bridged peptides: A new strategy for analysis

1993

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“…Although it has been suggested that STa needs to retain some toxicity in order to become immunogenic when carried by a carrier protein (3,35,36), other studies clearly indicated that nontoxic STa antigens in fusion formats elicited neutralizing antibodies (18,19,20,28,46). It was demonstrated that synthetic mutated pSTa (pSTa N11P , pSTa Y18N ), when chemically cross-linked to an LT B subunit or porcine IgG molecules, elicited anti-STa antibodies.…”

Section: Discussionmentioning

confidence: 99%

“…It was demonstrated that synthetic mutated pSTa (pSTa N11P , pSTa Y18N ), when chemically cross-linked to an LT B subunit or porcine IgG molecules, elicited anti-STa antibodies. Moreover, these anti-STa antibodies provided protection against ETEC infection (18,19,20). Data from the present study further confirm that the STa 13 toxoid, when fused to a carrier protein, elicits neutralizing anti-STa antibodies.…”

Section: Discussionmentioning

confidence: 99%

Heat-Labile- and Heat-Stable-Toxoid Fusions (LT _R192G -STa _P13F ) of Human Enterotoxigenic Escherichia coli Elicit Neutralizing Antitoxin Antibodies

et al. 2011

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Enterotoxigenic Escherichia coli (ETEC) strains, which colonize host small intestines and produce one or more enterotoxins, are a major cause of diarrheal disease (40). ETEC strains are responsible for hundreds of thousands of deaths each year worldwide, in addition to causing over one billion diarrheal episodes in immunocompromised individuals, international travelers, and deployed military personnel (14,33,38). The virulence determinants of ETEC in diarrhea disease are bacterial adhesins (colonization factor antigens [CFAs] and E. coli surface antigens) and enterotoxins known as heatlabile (LT) and heat-stable (ST) toxins (5,13,26,38,41). ETEC adhesins mediate initial bacterial attachment to host epithelial cells and subsequent colonization of small intestines. LT and ST type I (STa) enterotoxins disrupt fluid homeostasis and cause hypersecretion of fluid and electrolytes through activation of adenylate cyclase (by LT) or guanylate cyclase (by STa) in host small intestinal epithelial cells. Epidemiological and clinical studies indicated that approximately one-half of the ETEC strains isolated from diarrheal patients produce STa toxin only, one-quarter express LT toxin only, and one-quarter produce both toxins (13, 30,

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“…It is worth noting that the synthetic ST toxin used by Klipstein and colleagues was based on the STp sequence published by Chan and Giannella (5), which was later discovered to have two interchanged residues (STp, Asn11Tyr and Tyr18Asn) (54). However, this mutant ST peptide apparently had the same biological and immunological properties as native ST (16,27). In spite of the apparent successful generation of both a chemical conjugate and a synthetic ST vaccine candidate, these promising studies have not been further pursued.…”

Section: St Vaccinologymentioning

confidence: 99%

Heat-Stable Enterotoxin of EnterotoxigenicEscherichia colias a Vaccine Target

et al. 2010

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5Enterotoxigenic Escherichia coli (ETEC) is responsible for 280 million to 400 million episodes of diarrhea and about 380,000 deaths annually. Epidemiological data suggest that ETEC strains which secrete heat-stable toxin (ST), alone or in combination with heat-labile toxin (LT), induce the most severe disease among children in developing countries. This makes ST an attractive target for inclusion in an ETEC vaccine. ST is released upon colonization of the small intestine and activates the guanylate cyclase C receptor, causing profuse diarrhea. To generate a successful toxoid, ST must be made immunogenic and nontoxic. Due to its small size, ST is nonimmunogenic in its natural form but becomes immunogenic when coupled to an appropriate large-molecular-weight carrier. This has been successfully achieved with several carriers, using either chemical conjugation or recombinant fusion techniques. Coupling of ST to a carrier may reduce toxicity, but further reduction by mutagenesis is desired to obtain a safe vaccine. More than 30 ST mutants with effects on toxicity have been reported. Some of these mutants, however, have lost the ability to elicit neutralizing immune responses to the native toxin. Due to the small size of ST, separating toxicity from antigenicity is a particular challenge that must be met. Another obstacle to vaccine development is possible cross-reactivity between anti-ST antibodies and the endogenous ligands guanylin and uroguanylin, caused by structural similarity to ST. Here we review the molecular and biological properties of ST and discuss strategies for developing an ETEC vaccine that incorporates immunogenic and nontoxic derivatives of the ST toxin.

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Chemical synthesis of an octadecapeptide with the biological and immunological properties of human heat-stable Escherichia coli enterotoxin

Cited by 35 publications

References 25 publications

Disulfide structures of highly bridged peptides: A new strategy for analysis

Disulfide structures of highly bridged peptides: A new strategy for analysis

Heat-Labile- and Heat-Stable-Toxoid Fusions (LT _R192G -STa _P13F ) of Human Enterotoxigenic Escherichia coli Elicit Neutralizing Antitoxin Antibodies

Heat-Stable Enterotoxin of EnterotoxigenicEscherichia colias a Vaccine Target

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Chemical synthesis of an octadecapeptide with the biological and immunological properties of human heat-stable Escherichia coli enterotoxin

Cited by 35 publications

References 25 publications

Disulfide structures of highly bridged peptides: A new strategy for analysis

Disulfide structures of highly bridged peptides: A new strategy for analysis

Heat-Labile- and Heat-Stable-Toxoid Fusions (LT R192G -STa P13F ) of Human Enterotoxigenic Escherichia coli Elicit Neutralizing Antitoxin Antibodies

Heat-Stable Enterotoxin of EnterotoxigenicEscherichia colias a Vaccine Target

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Heat-Labile- and Heat-Stable-Toxoid Fusions (LT _R192G -STa _P13F ) of Human Enterotoxigenic Escherichia coli Elicit Neutralizing Antitoxin Antibodies