Outer Membrane Protein F (Porin) Preparation of Pseudomonas aeruginosa as a Protective Vaccine Against Heterologous Immunotype Strains in a Burned Mouse Model

Matthews-Greer, Janice; Gilleland, H. E.

doi:10.1093/infdis/155.6.1282

Cited by 93 publications

(88 citation statements)

References 29 publications

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“…Possession of the aerobactin system by pathogenic bacteria has been implicated as a virulence factor by epidemiological evidence (Montgomerie et al, 1984;Carbonetti et al, 1986;Linggood et al, 1987;Jacobson et al, 1988) and by studies using laboratory strains in experimental infections (Williams, 1979). We believe, however, that this paper contains the first report in which the aerobactin genes alone, isolated from other potential virulence factors encoded, for example, by ColV plasmids, have been studied in the genetic background of a clinical E. coli isolate.…”

Section: Discussionmentioning

confidence: 99%

“…Escherichia coli (O'Brien & Gibson, 1970) and other members of the Enterobacteriaceae (Pollock et al, 1970;Perry & San Clemente, 1979) synthesize the phenolic siderophore enterochelin (enterobactin), but some clinical isolates of enteric bacteria also possess a second high-affinity iron-uptake system mediated by the hydroxamate siderophore aerobactin (Braun, 1981 ;Warner et al, 1981 ;Roberts et al, 19866;Martinez et al, 1987). The ability to make and use aerobactin increased the virulence of E. coli K12 strains in experimental infections (Williams, 1979), and a number of epidemiological studies showed significantly higher incidence of the aerobactin system among bacteria isolated from extraintestinal infections than among isolates from the faeces of healthy individuals (Montgomerie et al, 1984;Carbonetti et al, 1986;Linggood et al, 1987;Jacobson et al, 1988).…”

Section: Introductionmentioning

confidence: 99%

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Inhibition of Biological Activities of the Aerobactin Receptor Protein in Rough Strains of Escherichia coli by Polyclonal Antiserum Raised against Native Protein

Roberts

Wooldridge²,

Gavine³

et al. 1989

Microbiology

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The aerobactin iron-uptake system of plasmid ColV-K30, genetically isolated from other plasmid determinants by molecular cloning, was sufficient to restore full virulence in a mouse peritonitis model to a clinical Escherichia coli isolate, D551 (078 : H-), whose resident aerobactin-encoding ColV plasmid had been lost by curing. Antiserum was raised in rabbits against live E. coli K 12 cells expressing the outer-membrane aerobactin receptor protein and absorbed with an isogenic strain lacking the receptor. This antiserum inhibited binding of aerobactin, cloacin DF13 and bacteriophage B74K to the native protein in whole E. coli K12 bacteria expressing the receptor, or in membranes prepared from such organisms. However, it did not react with the native receptor protein in several wild strains unless lipopolysaccharide was first removed by treatment with trichloroacetic acid, nor did it protect mice in experimental infections with strain D55 1. Antisera raised in rabbits against partially or fully denatured forms of the aerobactin receptor reacted only in assays involving denatured protein; they showed no inhibition of the biological activities of the native receptor.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Inhibition of Biological Activities of the Aerobactin Receptor Protein in Rough Strains of Escherichia coli by Polyclonal Antiserum Raised against Native Protein

Roberts

Wooldridge²,

Gavine³

et al. 1989

Microbiology

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“…In an attempt to overcome these problems some researchers have considered OMPs as immunotherapeutic agents, since they are non-toxic and are antigenically conserved among serotypes (Mutharia et al, 1982;Anwar et al, 1985). Gilleland et al (1 984) reported that antibodies to protein F offered protection against intraperitoneal challenge with laboratory strains of P. aeruginosa and, more recently, Matthews-Greer and Gilleland (1987) demonstrated protection with purified protein F against challenge with six heterologous LPS Fisher-Devlin immunotypes in a burned mouse model. The ability of IRMPs and other major OMPs, individually or in combination, to protect animals against challenge with different serotypes of P. aeruginosa remains to be investigated.…”

Section: Discussionmentioning

confidence: 99%

Antibody response to outer-membrane antigens of Pseudomonas aeruginosa in human burn wound infection

Ward

Anwar²,

Brown³

et al. 1988

Journal of Medical Microbiology

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Summary. There is little information about the local and systemic antibody response to surface antigens of bacteria growing in situ in infected lesions in man. In this study, Pseudomonas aeruginosa was obtained directly from the infected wounds of two patients with burns and studied without subculture. Outer-membrane proteins (OMPs) were investigated and compared with those of cells cultivated in the laboratory, with the aim of selecting defined growth conditions to give surface antigens more closely resembling those found in uivo. Several high-mol. wt (77 000-101 000) proteins were expressed in the outer membranes of the bacteria from the patients and could be phenotypically induced by cultivating the same isolate in irondepleted conditions in vitro. Other major OMPs (D, E, F, G and H) were also observed in cells taken from the lesions. Immunoblotting demonstrated that proteins D and E were recognised by different classes of immunoglobulins in the sera of both patients as was flagellar antigen present in the outer-membrane preparation of the P. aeruginosa from patient 1. Iron-regulated membrane proteins (IRMPs) were similarly detected, but more strongly by IgM from patient 1. Furthermore, a marked antibody response to IRMPs was noted at the site of infection. Bands of a similar intensity were seen after absorption of the sera with lipopolysaccharide (LPS) purified from the infecting strain. This indicated that the response observed was directed against OMPs (including IRMPs) and not against contaminating LPS.

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“…We have previously shown that active immunization with outermembrane (OM) protein F of P. aeruginosa affords protection from P. aeruginosa in a number of animal models, including a rat model of chronic pulmonary infection (Gilleland et al, 1988, a murine acute infection model (Gilleland et al, 1984) and a murine burn wound sepsis model (Matthews-Greer & Gilleland, 1987;Matthews-Greer et al, 1992). Since protein F purified from bacteria is not suitable for human vaccination due to its contamination with LPS and its requirement for detergent to prevent its denaturation into an insoluble precipitate, peptides of protein F, representing surface-exposed linear B cell epitopes, were identified and synthesized (Hughes et al, 1992 ;.…”

Section: Introductionmentioning

confidence: 99%

Pseudomonas aeruginosa outer-membrane protein F epitopes are highly immunogenic in mice when expressed on a plant virus

Brennan¹,

Jones²,

Gilleland

et al. 1999

Microbiology

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A synthetic peptide (peptide 10) representing a surface-exposed, linear B cell epitope from outer-membrane (OM) protein F of Pseudomonas aeruginosa was shown previously to afford protection in mice from P. aeruginosa infection. This peptide was expressed in tandem with the protein F peptide 18 on each of the two coat proteins of cowpea mosaic virus (CPMV). The chimaeric virus particles (CVPs) expressing the peptides on the S (small) coat protein (CPMV-PAE4) and L (large) coat protein (CPMV-PAE5) were used to immunize mice. Following subcutaneous immunization in Freund's and QuilA adjuvants, CPMV-PAE4 induced antibodies predominantly against peptide 18, whereas CPMV-PAE5 produced antibodies exclusively against peptide 10, indicating that the site of peptide expression on CPMV influences its immune recognition. The anti-peptide antibodies elicited by CPMV-PAE5 were predominantly of the IgG,, isotype, indicating a highly polarized THI-type response. The peptidespecific I gG, , strongly recognized the whole F protein, but more importantly, recognized protein F in all seven Fisher-Devlin immunotypes of P. aeruginosa. Furthermore, the peptide-specif ic IgG,, in CVP/QS-21 adjuvant-immunized mice was shown to bind complement and to augment phagocytosis of P. aeruginosa by human neutrophils in vitro. The ability of CPMV-PAE5 to induce P. aeruginosa-specif ic opsonic IgG,, gives it potential for further development as a protective vaccine against P. aeruginosa.

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Outer Membrane Protein F (Porin) Preparation of Pseudomonas aeruginosa as a Protective Vaccine Against Heterologous Immunotype Strains in a Burned Mouse Model

Cited by 93 publications

References 29 publications

Inhibition of Biological Activities of the Aerobactin Receptor Protein in Rough Strains of Escherichia coli by Polyclonal Antiserum Raised against Native Protein

Inhibition of Biological Activities of the Aerobactin Receptor Protein in Rough Strains of Escherichia coli by Polyclonal Antiserum Raised against Native Protein

Antibody response to outer-membrane antigens of Pseudomonas aeruginosa in human burn wound infection

Pseudomonas aeruginosa outer-membrane protein F epitopes are highly immunogenic in mice when expressed on a plant virus

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