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dc.contributor.authorBergin, David A
dc.contributor.authorReeves, Emer P
dc.contributor.authorMeleady, Paula
dc.contributor.authorHenry, Michael
dc.contributor.authorMcElvaney, Oliver J
dc.contributor.authorCarroll, Tomás P
dc.contributor.authorCondron, Claire
dc.contributor.authorChotirmall, Sanjay H
dc.contributor.authorClynes, Martin
dc.contributor.authorO'Neill, Shane J
dc.contributor.authorMcElvaney, Noel G
dc.date.accessioned2011-02-01T16:11:51Z
dc.date.available2011-02-01T16:11:51Z
dc.date.issued2010-12-01
dc.identifier.citationα-1 Antitrypsin regulates human neutrophil chemotaxis induced by soluble immune complexes and IL-8. 2010, 120 (12):4236-50 J. Clin. Invest.en
dc.identifier.issn1558-8238
dc.identifier.pmid21060150
dc.identifier.doi10.1172/JCI41196
dc.identifier.urihttp://hdl.handle.net/10147/120887
dc.description.abstractHereditary deficiency of the protein α-1 antitrypsin (AAT) causes a chronic lung disease in humans that is characterized by excessive mobilization of neutrophils into the lung. However, the reason for the increased neutrophil burden has not been fully elucidated. In this study we have demonstrated using human neutrophils that serum AAT coordinates both CXCR1- and soluble immune complex (sIC) receptor-mediated chemotaxis by divergent pathways. We demonstrated that glycosylated AAT can bind to IL-8 (a ligand for CXCR1) and that AAT-IL-8 complex formation prevented IL-8 interaction with CXCR1. Second, AAT modulated neutrophil chemotaxis in response to sIC by controlling membrane expression of the glycosylphosphatidylinositol-anchored (GPI-anchored) Fc receptor FcγRIIIb. This process was mediated through inhibition of ADAM-17 enzymatic activity. Neutrophils isolated from clinically stable AAT-deficient patients were characterized by low membrane expression of FcγRIIIb and increased chemotaxis in response to IL-8 and sIC. Treatment of AAT-deficient individuals with AAT augmentation therapy resulted in increased AAT binding to IL-8, increased AAT binding to the neutrophil membrane, decreased FcγRIIIb release from the neutrophil membrane, and normalization of chemotaxis. These results provide new insight into the mechanism underlying the effect of AAT augmentation therapy in the pulmonary disease associated with AAT deficiency.
dc.language.isoenen
dc.subjectGENETICSen
dc.subjectRESPIRATORY DISORDERen
dc.subject.meshADAM Proteins
dc.subject.meshAntigen-Antibody Complex
dc.subject.meshCase-Control Studies
dc.subject.meshChemotaxis, Leukocyte
dc.subject.meshGPI-Linked Proteins
dc.subject.meshHumans
dc.subject.meshInterleukin-8
dc.subject.meshMembrane Microdomains
dc.subject.meshMiddle Aged
dc.subject.meshModels, Immunological
dc.subject.meshMutation
dc.subject.meshNeutrophils
dc.subject.meshReceptors, IgG
dc.subject.meshReceptors, Interleukin-8A
dc.subject.meshRecombinant Proteins
dc.subject.meshalpha 1-Antitrypsin
dc.subject.meshalpha 1-Antitrypsin Deficiency
dc.titleα-1 Antitrypsin regulates human neutrophil chemotaxis induced by soluble immune complexes and IL-8.en
dc.typeArticleen
dc.contributor.departmentRespiratory Research Division, Department of Medicine, Royal College of Surgeons in Ireland, Education and Research Centre, Beaumont Hospital, Dublin, Ireland.en
dc.identifier.journalThe Journal of clinical investigationen
refterms.dateFOA2018-08-22T10:35:13Z
html.description.abstractHereditary deficiency of the protein α-1 antitrypsin (AAT) causes a chronic lung disease in humans that is characterized by excessive mobilization of neutrophils into the lung. However, the reason for the increased neutrophil burden has not been fully elucidated. In this study we have demonstrated using human neutrophils that serum AAT coordinates both CXCR1- and soluble immune complex (sIC) receptor-mediated chemotaxis by divergent pathways. We demonstrated that glycosylated AAT can bind to IL-8 (a ligand for CXCR1) and that AAT-IL-8 complex formation prevented IL-8 interaction with CXCR1. Second, AAT modulated neutrophil chemotaxis in response to sIC by controlling membrane expression of the glycosylphosphatidylinositol-anchored (GPI-anchored) Fc receptor FcγRIIIb. This process was mediated through inhibition of ADAM-17 enzymatic activity. Neutrophils isolated from clinically stable AAT-deficient patients were characterized by low membrane expression of FcγRIIIb and increased chemotaxis in response to IL-8 and sIC. Treatment of AAT-deficient individuals with AAT augmentation therapy resulted in increased AAT binding to IL-8, increased AAT binding to the neutrophil membrane, decreased FcγRIIIb release from the neutrophil membrane, and normalization of chemotaxis. These results provide new insight into the mechanism underlying the effect of AAT augmentation therapy in the pulmonary disease associated with AAT deficiency.


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