Your search keyword '"Geoffrey A. Stewart"' showing total 6 results

1. The immunobiology of allergenic peptidases

Author

Geoffrey A. Stewart and Clive Robinson

Subjects

Cockroach, biology, Peptide Hydrolases, biology.animal, Immunology, Immunology and Allergy, Environmental exposure, Microbiology

Published

2003

2. Cell lines of pulmonary and non-pulmonary origin as tools to study the effects of house dust mite proteinases on the regulation of epithelial permeability

Author

Clive Robinson, Philip J. Thompson, D.C. Gruenert, Mark B. Cannell, David R. Garrod, Geoffrey A. Stewart, Helen L Winton, and Hong Wan

Subjects

A549 cell, biology, Tight junction, Desmoplakin, Immunology, Cell junction, Epithelium, Cell biology, medicine.anatomical_structure, Cell culture, Permeability (electromagnetism), Extracellular, biology.protein, medicine, Immunology and Allergy

Abstract

Background Allergenic and non-allergenic proteinases from house dust mites (HDM) cause loss of adhesion between airway epithelial cells that may result in a loss of functional cohesion between the cells and thus assist in allergen presentation. Improved cellular assay systems are needed to ascertain the mechanisms involved. Objectives To survey a series of epithelial cell lines (Calu-3, 16HBE14o−, NCI-H292 and A549 from human airways, and MDCK from dog kidney) and establish their utility for studies of the effects of HDM proteinases from D. pteronyssinus on epithelial permeability. To develop an improved method for measuring changes in epithelial permeability induced by HDM proteinases and other provocants. Methods The permeability of epithelial monolayer cultures to mannitol was calculated from measurements of clearance using a technique that permits mathematical estimation and reduction of non-cellular diffusional constraints. Permeability was studied under control conditions and after perturbation of monolayers with HDM proteinases (separated into serine- and cysteine-proteinase classes) or chelation of extracellular Ca2+. Fluorescent antibody staining was used to investigate whether the cells expressed tight junctions (staining of ZO-1), desmosomes (staining of desmoplakin) and zonulae adherentes (staining of E-cadherin). Results The Calu-3 line was identified as an airway cell line that expressed functional tight junctions, desmosomes and zonulae adherentes. Calu-3 monolayers exhibited a low clearance and permeability to mannitol, similar to that seen in the extensively characterized MDCK cell line. Clearance and permeability were significantly increased by treatment with either HDM proteinase fraction or by calcium chelation. 16HBE14o− cells also had a low permeability to mannitol under control conditions and expressed a similar repertoire of functional proteins from major intercellular junctions. In contrast, NCI-H292 and A549 cell lines were functionally deficient in tight junctions, although they did express desmosomes and zonulae adherentes to a greater extent. Epithelial permeability was found to be a more appropriate and sensitive index of epithelial perturbation than was tracer clearance. Conclusion These results suggest that the Calu-3 and 16HBE14o− cell lines are useful tools in studying the mechanism of HDM proteinases on airway epithelial cell function. HDM proteinases of both cysteine and serine mechanistic classes were found to perturb epithelial adhesion and function.

Published

1998

3. On the potential significance of the enzymatic activity of mite allergens to immunogenicity. Clues to structure and function revealed by molecular characterization

Author

Geoffrey A. Stewart, Narayanaswamy Srinivasan, David R. Garrod, Clive Robinson, Noor Kalsheker, Philip J. Thompson, and Cecile King

Subjects

chemistry.chemical_classification, biology, Immunogenicity, Immunology, biology.organism_classification, medicine.disease_cause, Allergen, Enzyme, Antigen, Biochemistry, chemistry, Mite, medicine, Immunology and Allergy, Structure–activity relationship, Glycoprotein, Peptide sequence

Published

1997

4. The biochemistry of common aeroallergens

Author

Geoffrey A. Stewart and Philip J. Thompson

Subjects

business.industry, Immunology, Immunology and Allergy, Medicine, Physiology, Computational biology, business

Published

1996

5. Reduced platelet glutathione peroxidase activity and serum selenium concentration in atopic asthmatic patients

Author

Geoffrey A. Stewart, Philip J. Thompson, K. A. Powers, Neil L. A. Misso, and R. L. Gillon

Subjects

chemistry.chemical_classification, medicine.medical_specialty, Allergy, Antioxidant, business.industry, medicine.medical_treatment, Glutathione peroxidase, Immunology, Inflammation, medicine.disease, Atopy, Endocrinology, chemistry, Internal medicine, medicine, Immunology and Allergy, Platelet, medicine.symptom, business, Asthma, Whole blood

Abstract

Summary Background Asthmatic inflammation results in increased oxygen free radical generation and assessment of the activity of the selenitim (Se) dependent anti-oxidant enzyme, glutathione peroxidase (GSH-Px) in asthma may therefore be important. Objective To test the hypothesis that reduced GSH-Px activity and Se intake contribute to asthmatic infiammation, platelet and whole blood GSH-Px activities and serum and whole blood Se concentrations were measured and compared in atopic and non-atopic asthmatic patients and non-asthmatic control subjects. Methods GSH-Px activities of whole blood and isolated platelets were assessed in 41 asthmatic patients (33 atopic) and 41 age- and sex-matched non-asthmatic sttbjects (15 atopic) by spectrophotometric assay based oti the oxidation of NADPH. Se concentrations were determined by semi-automated fluorimetric assay. Results Mean (± sd) platelet GSH-Px activity was lower in asthmatic (89.5 ± 45.7 μmol NADPH oxidized min−1 g−1 of protein) than in non-asthmatic subjects (109,9 ± 41.9; P= 0.038) and in atopic (89.7 ± 45.1, n = 48) compared with non-atopie subiects (113.7 ± 40.9, n= 34: P= 0.016). Mean whole blood GSH-Px activity was also lower in atopic (12.2 ± 5.2 μmol NADPH oxidized min−1 g−1 of Hb) than in non-atopic subjects (14.5 ± 4.2; P= 0.038). In non-asthmatic subjects, the mean whole blood GSH-Px activity was lower in men (9.9 ± 3.5) than in women (14.5 ± 3.7; P = 0.0004) and was positively correlated with age (r= 0.51; P = 0.0006). Mean serum Se was lower in asthmatic (1.07 ± 0.12 μmol/L) than in non-asthmatic subjects (1.16 ± 0.31; P = 0.036), Using multiple linear regression, asthma was an independent predictor of decreased platelet GSH-Px after gender, age and serum Se were taken into account (P = 0.048) while atopy was a significant predictor of low whole blood GSH-Px independent of asthma, gender, age and whole blood Se (P = 0.033). Conclusions In addition to Se status, atopy, gender and uge all appear to influence GSH-Px activity, although the relative importance of these factors may difler in asthmatic and non-asthmatic populations. It seems likely that the reduced activity of this enzyme in platelets und hiood may reflect mechanisms associated with the pathogenesis and severity of asthma.

Published

1996

6. Differential expression of platelet activation markers in aspirin-sensitive asthmatics and normal subjects

Author

Geoffrey A. Stewart, Neil L. A. Misso, M.L. Taylor, and Philip J. Thompson

Subjects

Adult, Blood Platelets, Male, medicine.medical_specialty, P-selectin, Immunology, Population, Platelet Membrane Glycoproteins, Drug Hypersensitivity, Pathogenesis, chemistry.chemical_compound, Antigens, CD, Internal medicine, Humans, Immunology and Allergy, Medicine, Drug Interactions, Platelet, Platelet activation, Platelet Activating Factor, education, Aspirin, education.field_of_study, Arachidonic Acid, CD63, Platelet-activating factor, Tetraspanin 30, business.industry, Middle Aged, Flow Cytometry, Platelet Activation, Asthma, P-Selectin, Endocrinology, chemistry, Female, Collagen, business, Cell Adhesion Molecules, Platelet Aggregation Inhibitors, medicine.drug

Abstract

Summary Background Activation of platelets and expression of adhesion molecules (e.g. CD62P and CD63) which mediate interactions between platelets and other cells may be important in the pathogenesis of aspirin-sensitive asthma. Objective To determine the expression of CD62P and CD63 on platelets from aspirinsensitive asthmatic (ASA +), aspirin-tolerant asthmatic (ASA-) and normal subjects and to assess the modulatory effect of aspirin on platelet CD62P and CD63 expression following stimulation with either platelet-activating factor (PAF), arachidonic acid (AA) or collagen (COL). Methods Platelet-rich plasma was obtained from 10 ASA +, 10 ASA—and 10 normal control subjects, and expression of CD62P and CD63 was measured by flow cytometry. Platelets were stimulated with PAF (10, 80 nM), AA (0.1, 1 mM) or COL (80, 800 μg/mL) with or without aspirin (concentration range 0.4–4 mg/mL). Results In the absence of aspirin, CD62P expression induced by AA and COL was greater in ASA+ patients compared with control subjects (P

Published

1996