Enhanced expression of high-affinity IgE receptor (Fc epsilon RI) a chain in human allergen-induced rhinitis with co-localization to mast cells, macrophages, eosinophils, and dendritic cells
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作者:
Rajakulasingam, K
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Rajakulasingam, K
Durham, SR
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Durham, SR
OBrien, F
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
OBrien, F
Humbert, M
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Humbert, M
Barata, LT
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Barata, LT
Reece, L
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Reece, L
Kay, AB
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Kay, AB
Grant, JA
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机构:HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
Grant, JA
机构:
[1] HOP ANTOINE BECLERE, SERV PNEUMOL, CLAMART, FRANCE
[2] UNIV TEXAS, MED BRANCH, DEPT ALLERGY & IMMUNOL, GALVESTON, TX 77550 USA
Background: IgE-dependent activation of mast cells and basophils through the high-affinity IgE receptor (Fc epsilon RI) is involved in the pathogenesis of allergen-induced immediate and late responses. Objective: We investigated the expression and cellular distribution of Fc epsilon RI in the nasal mucosa after allergen challenge in patients with summer hay fever. Methods: Fourteen grass pollen-sensitive patients and seven normal control subjects underwent nasal challenge with grass pollen and allergen diluent in random order separated by 2 weeks. Nasal airway caliber was monitored by acoustic rhinometry, and nasal biopsy was performed at 6 hours. Messenger RNA for Fc epsilon RI was determined by using reverse-transcription polymerase chain reaction, and Fc epsilon RI protein-expression was determined by immunohistology with a mouse monoclonal antibody (22E7) and a rabbit polyclonal antibody (997) directed against the or subunit. Co-localization of Fc epsilon RI receptors was performed by using double-immunostaining methods. Results: In atopic subjects, there was a significant early decrease in nasal airway caliber, which extended up to 6 hours after allergen challenge. Fc epsilon RI mRNA levels were elevated at 6 hours (p = 0.03). Cells expressing Fc epsilon RI protein were increased in patients with atopic rhinitis compared with normal control subjects (p = 0.03). Further increases in Fc epsilon RI+ cells were observed after allergen challenge only in the atopic group (p = 0.02). Double immunohistochemistry revealed that the majority of Fc epsilon RI+ cells were mast cells (64%), followed by macrophages (20%), eosinophils (4%), and dendritic cells (2%), with 10% Fc epsilon RI+ cells being unidentified. Conclusions: Our results demonstrate increased Fc epsilon RI expression during allergen induced rhinitis and highlight a potential target for treatment.
机构:
NIAID, Lab Allerg Dis, NIH, Bethesda, MD 20892 USANorth Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USA
Yin, Yuzhi
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Fukuyama, Tomoki
Desai, Avanti
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机构:
NIAID, Lab Allerg Dis, NIH, Bethesda, MD 20892 USANorth Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USA
Desai, Avanti
Arthur, Greer K.
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North Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USANorth Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USA
Arthur, Greer K.
Baumer, Wolfgang
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North Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USANorth Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USA
Baumer, Wolfgang
Beaven, Michael A.
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NHLBI, Lab Mol Immunol, NIH, Bethesda, MD 20892 USANorth Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USA
Beaven, Michael A.
Metcalfe, Dean D.
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NIAID, Lab Allerg Dis, NIH, Bethesda, MD 20892 USANorth Carolina State Univ, Coll Vet Med, Dept Mol Biomed Sci, Raleigh, NC 27607 USA