Modulation of β1-integrins on hemopoietic progenitor cells after allergen challenge in asthmatic subjects

Mobilization of hemopoietic progenitor cells from the bone marrow (BM) is a feature of inflammatory asthmatic responses. Understanding the mechanisms regulating progenitor cell mobilization and trafficking to the peripheral circulation might be important for the development of effective asthma thera...

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Published inJournal of allergy and clinical immunology Vol. 122; no. 4; pp. 803 - 810
Main Authors Catalli, Adriana E., Thomson, Jennifer V., Babirad, Irene M., Duong, MyLinh, Doyle, Tracey M., Howie, Karen J., Newbold, Paul, Craggs, Richard I., Foster, Martyn, Gauvreau, Gail M., O'Byrne, Paul M., Sehmi, Roma
Format Journal Article
LanguageEnglish
Published New York, NY Elsevier Inc 01.10.2008
Elsevier
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ISSN0091-6749
DOI10.1016/j.jaci.2008.07.021

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Abstract Mobilization of hemopoietic progenitor cells from the bone marrow (BM) is a feature of inflammatory asthmatic responses. Understanding the mechanisms regulating progenitor cell mobilization and trafficking to the peripheral circulation might be important for the development of effective asthma therapies. We investigated the role of adhesion molecules in the mobilization of hemopoietic progenitor cells from the BM during an allergen-induced asthmatic response. BM and peripheral blood samples were obtained from dual-responders with mild asthma before and at several time points after allergen challenge. Fluctuations in expression and adhesive properties of β1- and β2-integrins on CD34+CD45+ progenitor cells were assessed by using flow cytometry and adhesion to protein-coated wells, respectively. On BM-derived CD34+CD45+ cells, expression of very late antigen (VLA) 4, but not VLA-5 or Mac-1, decreased significantly 24 hours after allergen challenge and had begun to recover by 48 hours after challenge. In peripheral blood allergen challenge induced a significant decrease in VLA-4 levels after 6 hours, which had not recovered by 96 hours after challenge. Similarly, VLA-5 expression decreased, most prominently at 72 to 96 hours after allergen challenge. In contrast, Mac-1 levels did not change. Chemokine-stimulated adhesion of BM-derived CD34+CD45+ cells to fibronectin was significantly attenuated 24 hours after challenge. Furthermore, adhesion to fibronectin and vascular cell adhesion molecule 1 was greatly reduced by anti-VLA-4 or anti-VLA-5 antibodies. Preferential downregulation of β1-integrin expression on progenitor cells can reduce the tethering forces to BM components, thus facilitating their egress to the peripheral circulation during an allergic inflammatory response.
AbstractList Mobilization of hemopoietic progenitor cells from the bone marrow (BM) is a feature of inflammatory asthmatic responses. Understanding the mechanisms regulating progenitor cell mobilization and trafficking to the peripheral circulation might be important for the development of effective asthma therapies. We investigated the role of adhesion molecules in the mobilization of hemopoietic progenitor cells from the BM during an allergen-induced asthmatic response. BM and peripheral blood samples were obtained from dual-responders with mild asthma before and at several time points after allergen challenge. Fluctuations in expression and adhesive properties of β1- and β2-integrins on CD34+CD45+ progenitor cells were assessed by using flow cytometry and adhesion to protein-coated wells, respectively. On BM-derived CD34+CD45+ cells, expression of very late antigen (VLA) 4, but not VLA-5 or Mac-1, decreased significantly 24 hours after allergen challenge and had begun to recover by 48 hours after challenge. In peripheral blood allergen challenge induced a significant decrease in VLA-4 levels after 6 hours, which had not recovered by 96 hours after challenge. Similarly, VLA-5 expression decreased, most prominently at 72 to 96 hours after allergen challenge. In contrast, Mac-1 levels did not change. Chemokine-stimulated adhesion of BM-derived CD34+CD45+ cells to fibronectin was significantly attenuated 24 hours after challenge. Furthermore, adhesion to fibronectin and vascular cell adhesion molecule 1 was greatly reduced by anti-VLA-4 or anti-VLA-5 antibodies. Preferential downregulation of β1-integrin expression on progenitor cells can reduce the tethering forces to BM components, thus facilitating their egress to the peripheral circulation during an allergic inflammatory response.
Background Mobilization of hemopoietic progenitor cells from the bone marrow (BM) is a feature of inflammatory asthmatic responses. Understanding the mechanisms regulating progenitor cell mobilization and trafficking to the peripheral circulation might be important for the development of effective asthma therapies. Objective We investigated the role of adhesion molecules in the mobilization of hemopoietic progenitor cells from the BM during an allergen-induced asthmatic response. Methods BM and peripheral blood samples were obtained from dual-responders with mild asthma before and at several time points after allergen challenge. Fluctuations in expression and adhesive properties of β1- and β2-integrins on CD34+ CD45+ progenitor cells were assessed by using flow cytometry and adhesion to protein-coated wells, respectively. Results On BM-derived CD34+ CD45+ cells, expression of very late antigen (VLA) 4, but not VLA-5 or Mac-1, decreased significantly 24 hours after allergen challenge and had begun to recover by 48 hours after challenge. In peripheral blood allergen challenge induced a significant decrease in VLA-4 levels after 6 hours, which had not recovered by 96 hours after challenge. Similarly, VLA-5 expression decreased, most prominently at 72 to 96 hours after allergen challenge. In contrast, Mac-1 levels did not change. Chemokine-stimulated adhesion of BM-derived CD34+ CD45+ cells to fibronectin was significantly attenuated 24 hours after challenge. Furthermore, adhesion to fibronectin and vascular cell adhesion molecule 1 was greatly reduced by anti-VLA-4 or anti-VLA-5 antibodies. Conclusions Preferential downregulation of β1-integrin expression on progenitor cells can reduce the tethering forces to BM components, thus facilitating their egress to the peripheral circulation during an allergic inflammatory response.
Author Gauvreau, Gail M.
Catalli, Adriana E.
O'Byrne, Paul M.
Duong, MyLinh
Howie, Karen J.
Babirad, Irene M.
Foster, Martyn
Craggs, Richard I.
Newbold, Paul
Thomson, Jennifer V.
Sehmi, Roma
Doyle, Tracey M.
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IsPeerReviewed true
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Issue 4
Keywords allergen
mobilization
LFA
asthma
VLA
BM
Adhesion
egress
VCAM
integrins
PB
fibronectin
SDF
inflammation
vascular cell adhesion molecule 1
SMFI
Stromal cell–derived factor
Vascular cell adhesion molecule
Leukocyte function–associated antigen
Specific mean fluorescence intensity
peripheral blood
Very late antigen
Bone marrow
Human
Lung disease
Allergy
Immunopathology
Vascular cell adhesion molecule 1
Respiratory disease
Stem cell
Cell adhesion molecule
Inflammation
Fibronectin
Asthma
Mobilization
Immunology
β1 integrin
Modulation
Bronchus disease
Obstructive pulmonary disease
Allergen
Provocation test
Language English
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SSID ssj0009389
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Snippet Mobilization of hemopoietic progenitor cells from the bone marrow (BM) is a feature of inflammatory asthmatic responses. Understanding the mechanisms...
Background Mobilization of hemopoietic progenitor cells from the bone marrow (BM) is a feature of inflammatory asthmatic responses. Understanding the...
SourceID pascalfrancis
crossref
elsevier
SourceType Index Database
Enrichment Source
Publisher
StartPage 803
SubjectTerms Adhesion
allergen
Allergy and Immunology
asthma
Biological and medical sciences
egress
fibronectin
Fundamental and applied biological sciences. Psychology
Fundamental immunology
inflammation
integrins
Medical sciences
mobilization
Sarcoidosis. Granulomatous diseases of unproved etiology. Connective tissue diseases. Elastic tissue diseases. Vasculitis
vascular cell adhesion molecule 1
Title Modulation of β1-integrins on hemopoietic progenitor cells after allergen challenge in asthmatic subjects
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https://www.clinicalkey.es/playcontent/1-s2.0-S009167490801350X
https://dx.doi.org/10.1016/j.jaci.2008.07.021
Volume 122
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