Search

Your search keyword '"Relf, W. A."' showing total 12 results
Start Over Author "Relf, W. A."
12 results on '"Relf, W. A."'

3. Sensitivity to ultraviolet radiation in a dominantly inherited form of xeroderma pigmentosum.

Author

Imray, F P, Hockey, A, Relf, W, Ramsay, R G, and Kidson, C

Abstract

An Australian family is described in which a mild form of xeroderma pigmentosum (XP) is inherited as an autosomal dominant trait. Studies of lymphoblastoid cells and fibroblasts from affected persons demonstrated cellular sensitivity to ultraviolet (UV) light as judged by diminished clonogenicity and higher frequencies of UV induced chromosome aberrations compared to normal controls. After UV irradiation of dominant XP cells, replicative DNA synthesis was depressed to a greater extent than normal and the level of UV induced DNA repair synthesis was lower than that in normal cells. The level of sister chromatid exchanges and the numbers of 6-thioguanine resistant mutants induced by UV irradiation were equal to those found in normal controls. Although two subjects in the family had skin cancers, this dominant form of XP is not apparently associated with high risk, or large numbers, of skin cancers in affected persons. [ABSTRACT FROM PUBLISHER]

Published
1986

4. Mapping the minimal murine T cell and B cell epitopes within a peptide vaccine candidate from the conserved region of the M protein of group A streptococcus.

Author

Hayman, W A, Brandt, E R, Relf, W A, Cooper, J, Saul, A, and Good, M F

Abstract

The highly conserved C-terminus of the M protein of group A streptococcus (GAS) is a promising vaccine candidate. An epitope within the conserved C-terminus of the M protein, peptide 145 (a 20-mer with the sequence: LRRDLDASREAKKQVEKALE), has been defined which is the target of opsonic antibodies in both humans and mice, and is recognized by the sera of most adults living in areas of high streptococcal exposure. However, due to potential cross-reactivity between T cells stimulated by this region of the M protein and host cardiac myosin, it is critical to define precisely the minimal protective epitopes within p145. Studies have shown that the immunodominant epitope expressed by p145 is conformational, occurring as an alpha-helical coiled-coil. To enable us to map the murine minimal B cell and T cell epitopes within p145, we have used a novel strategy that allowed us to present shorter sequences of p145 in a native-like conformation. The minimal B cell epitope was found to be contained within residues 7-20 of the p145 sequence, and we have shown that mice immunized with this region are able to generate antibodies that bind to and also opsonize the organism GAS. The T cell epitope is located at the N-terminal region of the p145 sequence, residues 3-14. We have managed, therefore, to define a vaccine candidate--a minimal opsonic B cell epitope within the p145 sequence--that does not incorporate a potentially deleterious T cell epitope. [ABSTRACT FROM AUTHOR]

Published
1997
Full Text
View/download PDF

5. Protective and nonprotective epitopes from amino termini of M proteins from Australian aboriginal isolates and reference strains of group A streptococci.

Author

Brandt, E R, Teh, T, Relf, W A, Hobb, R I, and Good, M F

Abstract

The M protein is the primary vaccine candidate to prevent group A streptococcal (GAS) infection and the subsequent development of rheumatic fever (RF). However, the large number of serotypes have made it difficult to design a vaccine against all strains. We have taken an approach of identifying amino-terminal M protein epitopes from GAS isolates that are highly prevalent in GAS-endemic populations within the Northern Territory (NT) of Australia. Australian Aboriginals in the NT experience the highest incidence of RF worldwide. To develop a vaccine for this population, 39 peptides were synthesized, representing the amino-terminal region of the M protein from endemic GAS. Mice immunized with these peptides covalently linked to tetanus toxoid and emulsified in complete Freund's adjuvant raised high-titer antibodies. Over half of these sera reduced bacterial colony counts by >80% against the homologous isolate of GAS. Seven of the peptide antisera also cross-reacted with at least three other heterologous peptides by enzyme-linked immunosorbent assay. Antiserum to one peptide, BSA10(1-28), could recognize six other peptides, and five of these peptides could inhibit opsonization mediated by BSA10(1-28) antiserum. Cross-opsonization studies showed that six of these sera could opsonize at least one heterologous isolate of GAS. These data reveal vaccine candidates specific to a GAS-endemic area and show the potential of some to cross-opsonize multiple isolates of GAS. This information will be critical when considering which epitopes may be useful in a multiepitope vaccine to prevent GAS infection.

Published
2000

6. Antibody detection ELISAS for malaria diagnosis

Author

Patricia Graves, Boreham, R., Robert, G., Fray, L., Xu, L. J., Huang, Y. M., Relf, W., Saul, A., and Kidson, C.

Subjects
Immunoglobulin M, Evaluation Studies as Topic, Immunoglobulin G, Molecular Sequence Data, Malaria, Vivax, Antibodies, Monoclonal, Humans, Antigens, Protozoan, Enzyme-Linked Immunosorbent Assay, Amino Acid Sequence, Malaria, Falciparum, Sensitivity and Specificity, Antibodies, Anti-Idiotypic
Abstract

Parasite extracts of Plasmodium falciparum and P. chabaudi and three synthetic peptides from the P. falciparum MSA2 merozoite antigen were tested for suitability as antigens in an antibody detection ELISA using sera from malaria patients in Brisbane. The P. chabaudi extract was superior to P. falciparum extract for detecting P. vivax cases, while for P. falciparum cases the two parasite extracts were equivalent. Single peptide antigens were generally less sensitive than parasite extracts; however, peptides G3 and G7 were more sensitive than parasite extracts in detecting first attacks of P. vivax. Examination of isotype specific responses demonstrated that this may be explained by higher IgG responses to these peptides in first than in subsequent P. vivax attacks. Because of the differing antibody specificities in primary and secondary P. falciparum and P. vivax cases, the best sensitivity was achieved by using the combined results of assays with three antigens: P. chabaudi, peptide G3 and peptide G7. The combined sensitivity was 77.1% for P. falciparum and 88.6% for P. vivax acute cases with 91.1% specificity.

9. Mapping a conserved conformational epitope from the M protein of group A streptococci.

Author

Relf WA, Cooper J, Brandt ER, Hayman WA, Anders RF, Pruksakorn S, Currie B, Saul A, and Good MF

Subjects
Animals, Humans, Mice, Amino Acid Sequence, Antibodies, Bacterial immunology, Circular Dichroism, Conserved Sequence, Mice, Inbred Strains, Molecular Sequence Data, Protein Conformation, Protein Structure, Secondary, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins immunology, Rheumatic Fever microbiology, Trifluoroethanol, Antigens, Bacterial chemistry, Bacterial Outer Membrane Proteins, Bacterial Proteins chemistry, Bacterial Proteins immunology, Carrier Proteins, Epitopes chemistry, Peptide Mapping, Streptococcus pyogenes immunology
Abstract

The carboxyl terminus of the M protein of group A streptococci (GAS) is highly conserved and contains epitopes that have been shown to induce opsonic antibodies and protection against GAS infection. This region of the protein can also stimulate T cells, which can react in vitro with heart antigens. Since different segments of the carboxyl terminus may be involved in immunity to GAS and in the pathogenesis of autoimmune disease (rheumatic heart disease), it is important to precisely define critical epitopes. However, the M protein is known to be a coiled coil, and a critical immunodominant antibody-binding epitope within this region (peptide 145, a 20-mer with the sequence LRRDLDASREAKK-QVEKALE) is shown here to be conformational. Thus, small synthetic overlapping peptides of 8-12 amino acids in length that span peptide 145 (p145) were unable to capture antibodies present in p145-immune mouse sera or in endemic human sera, even though antibodies raised to these small peptides coupled to diphtheria toxoid could bind the smaller peptides and, in some cases, p145. A series of mutated peptides in which every residue of p145 was sequentially altered also failed to identify critical residues for antibody binding. We thus devised a strategy to produce chimeric peptides in which small peptides copying the M protein sequence were displayed within a larger 28-mer peptide derived from the sequence of the GCN4 leucine zipper DNA binding protein of yeast. A 12-amino-acid window of the p145 sequence was inserted into the GCN4 peptide in such a way as to preserve any potential helical structure. The window was moved along one residue at a time to give a series of peptides representing p145. Circular dichroism demonstrated that these larger chimeric peptides and p145, but not a shorter 12-mer peptide, displayed alpha-helical potential in 50% trifluoroethanol. Certain chimeric peptides efficiently captured antibodies specific for p145 and thus enabled us to map the minimal antibody-binding sequence. RRDLDASREAKK, referred to as J(1)2. The chimeric peptide containing this sequence, referred to as J2, was able to inhibit opsonization of GAS by human antisera containing anti-peptide 145 antibodies. The T-cell response from p145-immunized responder B10.BR mice to J2 and J(I)2 was much lower than the response to p145 and mapped to a different peptide.

Published
1996

10. Imported malaria in Australia.

Author

Boreham RE and Relf WA

Subjects
Antimalarials therapeutic use, Humans, Malaria, Falciparum prevention & control, Malaria, Vivax prevention & control, New South Wales epidemiology, Queensland epidemiology, Recurrence, Retrospective Studies, Malaria, Falciparum epidemiology, Malaria, Vivax epidemiology, Travel
Abstract

Objective: To obtain information on imported malaria in Australia., Design and Setting: Patients with malaria diagnosed by microscopy by laboratories in southeast Queensland and northern New South Wales between October 1987 and December 1988 were included in this study. The chi 2 test was used to analyse data., Patients: Blood films, details of prophylactic regimens and clinical history were received from 146 patients., Main Outcome Measures: This study was to determine the percentage of patients infected with each malaria species, where they contracted their infections, whether they had taken appropriate prophylactic agents and to determine the relationship between parasitaemia and previous exposure, symptoms and prophylaxis., Results: One hundred patients (68.5%) had Plasmodium vivax malaria and 33 patients (22.6%) had Plasmodium falciparum malaria, with 3 (2.1%) infected with both of these malaria species. Ten cases (6.8%) were presumptively diagnosed as infections but diagnosis by microscopy was uncertain. Seventy-four per cent of the P. vivax infections and 85% of the P. falciparum infections were contracted in Papua New Guinea. Patients presented with a range of blood parasite concentrations that did not correlate with their symptoms, previous infection with malaria (P greater than 0.25) or the regular taking of prophylactic drugs (P greater than 0.1). Only 41% of the patients took any prophylactic drugs; the figure for temporary visitors to malarious areas was 54%. Only 11.6% of patients were taking the recommended drugs for the malarious areas they visited or were resident in., Conclusions: Constant monitoring of malarial infections is needed to ensure that appropriate advice is given to the traveller. Our study supports the dogma that malaria should be suspected in all patients who have been to malarious areas, regardless of previous malarious attacks, prophylaxis, treatment or the time which has elapsed since leaving the area.

Published
1991
Full Text
View/download PDF

11. Limited repertoire of the C-terminal region of the M protein in Streptococcus pyogenes.

Author

Relf WA and Sriprakash KS

Subjects
Electrophoresis, Agar Gel, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length, Antigens, Bacterial, Bacterial Outer Membrane Proteins genetics, Bacterial Proteins genetics, Carrier Proteins, Streptococcus pyogenes genetics
Abstract

We have amplified genomic sequences (emm) that may encode M protein from strains of Streptococcus pyogenes using the polymerase chain reaction (PCR). Genomic DNA from 22 isolates representing 14 M serotypes was selected for the study. Primers which corresponded to the observed N-terminal signal sequence and the variable C-terminal sequences of emm6, emm49 and ennX were used. PCR products using emm6 and emm49 oligonucleotides were classified into two mutually exclusive groups which correspond to the presence or absence of serum opacity factor. These findings support the concept of limited heterogeneity in the C-terminal sequences of the M protein.

Published
1990
Full Text
View/download PDF

12. Diagnosis of Plasmodium vivax malaria using a specific deoxyribonucleic acid probe.

Author

Relf WA, Boreham RE, Tapchaisri P, Khusmith S, Healey A, Upcroft P, Tharavanij S, and Kidson C

Subjects
Animals, Base Sequence, Blotting, Southern, DNA, Protozoan analysis, Humans, Malaria parasitology, Molecular Sequence Data, Nucleic Acid Hybridization, Plasmodium falciparum isolation & purification, DNA Probes, Malaria diagnosis, Plasmodium vivax isolation & purification
Abstract

A deoxyribonucleic acid (DNA) probe which specifically distinguishes Plasmodium vivax from P. falciparum malaria has been derived from a P. vivax genomic DNA library. This probe, VPL101, consists of 3.2 kilobase pairs and does not hybridize with up to 6 micrograms of human or P. falciparum DNA. VPL101 contains at least two copies of a 205 base pair repeat sequence. The subcloned repeat probe, VPL101/5, reacted with 73 of 76 microscopically diagnosed P. vivax samples but not with any of 17 human DNA samples or any of 8 P. falciparum DNA samples from cultured parasites. It was possible to detect P. vivax in mixed infections in which only P. falciparum parasites were identifiable by microscopy. This P. vivax DNA probe provides a useful epidemiological tool for malaria control programmes.

Published
1990
Full Text
View/download PDF

Catalog

Books, media, physical & digital resources
See catalog results