 RI)
Receptor- Chain mRNA and Protein-bearing Eosinophils
in Human Allergen-induced Atopic Asthma
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ABSTRACT |
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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Fc
RI receptors play an important role in allergen-induced mediator release and antigen presentation
by mast cells, basophils, and monocyte/macrophages in atopic disorders. The expression of FcRI by
tissue eosinophils in atopic asthma after allergen challenge has not been established. For this reason
we attempted to identify mRNA and protein product + FcRI
eosinophils in cytospins made from
bronchoalveolar lavage (BAL) from atopic asthmatics (n = 9) and nonatopic normal subjects (n = 4)
24 h after segmental challenge with allergen or diluent. Messenger RNA for FcRI was determined
using in situ hybridization and FcRI protein expression by immunocytochemistry using a mouse
monoclonal antibody 22E7. Colocalization of FcRI receptors to eosinophils was performed using
chromotrope 2R. When compared with a control challenge, segmental challenge with Dermatophagoides pteronyssinus induced significant BAL eosinophilia (p = 0.007). The total number of BAL FcRI
mRNA and protein-positive cells also increased in asthmatics, median values 2 (0.7-7.2) and 11.5 (0.6-65.0) × 106 cells (p = 0.02) and 0 (0-0.3 × 106) and 3.1 × 106 (0.45 
162.5 × 106) cells (p = 0.007), respectively, for mRNA and protein. Net increases in FcRI+ cells correlated with the net increases in BAL eosinophils (r = 0.98, p = 0.0001 for mRNA and r = 0.72, p = 0.02 for protein). Colocalization studies with chromotrope 2R revealed that only 4% of FcRI+ cells were eosinophils after
control challenge and, in contrast, 85 to 95% of FcRI+ cells were eosinophils after allergen. There
were no differences in the numbers of FcRI+ cells or eosinophils in normal control subjects. Our results demonstrated that local endobronchial allergen provocation in atopic asthmatics results in increased synthesis and expression of FcRI predominantly on BAL eosinophils.
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Asthma is characterized by mucosal inflammation of the airways and is closely related to atopy, which is characterized by enhanced IgE responses to common environmental allergens.
Epidemiologic studies link total serum IgE concentrations
with the incidence of asthma symptoms and bronchial hyperresponsiveness (1, 2). An important characteristic of IgE is its
ability to bind to mast cells and basophils with high affinity
through its Fc portion to the IgE receptor (Fc RI) (3, 4).
FcRI comprises an chain, a 
chain, and two disulphide-linked 
chains. Alpha chain is involved in IgE binding and receptor internalization, resulting in the allergic mediator release process, whereas chain plays a role in signal transduction (3, 4). Cross-linking of the Fc RI, even in the absence of
IgE, results in mast-cell triggering (5). In sensitized persons,
the interaction of FcRI-bound IgE with the relevant antigen
elicits an immediate reaction characterized by mast-cell degranulation and release of preformed mediators and cytokines.
Apart from mediating the immediate response, the allergen-induced late phase skin reaction (LPR) has also been
shown to be IgE-dependent (6, 7). Biopsies of allergen-induced
cutaneous late phase reactions have demonstrated IgE-bound
antigen-presenting cells such as epidermal Langerhans' cells
and dermal dendritic cells (8, 9). More recently, it has been
demonstrated that Langerhans' cells (10, 11), dermal dendritic
cells (10, 12), peripheral blood monocytes (13), and eosinophils (14) may all express the high affinity receptor for IgE
(FcRI). FcRI, therefore, is being considered as a critical
component of the effector arm of the allergic response in mediating both early and late phase responses. We have recently
demonstrated elevated numbers of FcRI+ cells in the bronchial submucosa of patients with stable, mild asthma compared with control subjects (17). Colocalization studies revealed that the majority of FcRI+ cells were identified as
mast cells and macrophages and a much smaller percentage
were eosinophils. However, a variable proportion (0 to 40%)
of these eosinophils were FcRI+. Because of the relatively small numbers of eosinophils in this baseline study, we felt it important to reevaluate expression of Fc RI by bronchial
eosinophils after allergen challenge.
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METHODS |
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Patients
Nine patients (four male and five female) with a history of house-dust-mite-sensitive asthma and four nonatopic, normal subjects (three male and one female) took part in the study (Table 1). Subjects were recruited from the Allergy Clinic and from the general public after an advertisement in the local newspaper. All subjects were nonsmokers. Asthmatic subjects were chosen on the basis of (1) a clear history of asthma symptoms, (2) histamine PC20 value of < 16.0 mg/ml in the previous 2 wk, (3) a strongly positive skin weal response (> 5 mm) to prick testing with Dermatophagoides pteronyssinus extract (Soluprick; ALK, Horsholm, Denmark), and (4) positive RAST test for the same house dust mite extract (Table 1). Normal volunteers were asymptomatic, had negative skin responses to a panel of 11 common aeroallergens, including house dust mite, animal danders, moulds, and grass pollen (Soluprick; ALK), and negative RAST tests for the same panel of allergen extracts. None of the subjects was receiving oral steroids or theophylline preparations during the previous 6 mo, and inhaled steroids were withheld for 72 h prior to the study. None of the subjects had a history of lower respiratory tract infection in the preceding 4 wk or of any current medical illness other than atopic asthma. Subjects with FEV1 of less than 80% predicted and histamine PC20 < 1.0 mg/ml were excluded. None of the patients had received immunotherapy in the previous 5 yr. The study was approved by the Ethics Committee of the Royal Brompton National Heart and Lung Hospital, London, and informed written consent was obtained from each subject.
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Study Design
Subjects were asked to attend the laboratory to undergo two fiberoptic bronchoscopies separated by 24 h. Fiberoptic bronchoscopy was undertaken as previously described (17). In brief, all subjects received nebulized albuterol (2.5 mg) and intravenous atropine (0.6 mg) and midazolam (0 to 10 mg) 10 min prior to the procedure. Oxygen was delivered via the nasal canulae throughout the procedure, and oxygen saturation was monitored by pulse oximetry. Local anaesthesia of the upper airways was induced with 2 to 4% lidocaine. The bronchoscope (BFP20; Olympus Corp., Lake Success, NY) was then passed through the nares or mouth, and as much as 10 ml of lidocaine were introduced through the bronchoscope to anaesthetize the vocal cords and lower airways. After inspection of the bronchial tree, the bronchoscope was wedged in the lateral subsegment of the right middle lobe to undertake a control challenge with 5 ml of sterile saline solution prewarmed to 37° C. The bronchoscope was then passed into the lateral subsegment of lingula of the left lung, and 5 ml of prewarmed saline containing 100 BU of allergen (Der p) were instilled. Allergen and control challenge sites were randomly chosen for individual subjects. The appearance of the airways was then observed for 5 min. If there was no visible reaction to 100 BU of allergen, a further 5 ml of saline containing 400 BU of allergen were then instilled into the allergen challenge site and was observed for 5 min to confirm an airway response (18). The subjects were then observed closely, and a second bronchoscopy was performed with the same premedications and oxygenation at 24 h after segmental allergen challenge. After inspection of the bronchial tree, BAL was performed using 120 ml of prewarmed 0.9% saline solution at each challenge site. All subjects were then observed closely for 2 h.
Processing of Bronchoalveolar Lavage Fluid
BAL fluid was passed through two layers of sterile gauze to remove
debris and then centrifuged at 500 × g for 10 min at 4° C. The pellet
was then resuspended in RPMI 1640 (Chester Beatty Laboratories,
London, UK) supplemented with 2 U/ml sodium heparin. The fluid
was then centrifuged again at 500 × g for 10 min. The cells were then
resuspended at 0.25 to 0.5 × 106 cells/ml in RPMI-1640 medium
(GIBCO, Paisley, UK) supplemented with 100 IU/ml penicillin/streptomycin (GIBCO), 2 mM L-glutamine (GIBCO), and 5% human AB
serum (Sigma, Poole, Dorset, UK); 100 µl of cells were used per poly-
L-lysine-coated slide and mounted on Shandon 190005 filter cards and
then centrifuged in a Shandon 2 machine for 5 min at 500 rpm (Shandon Ltd, Runcorn, Cheshire, UK). Slides were then air-dried and
fixed in 4% paraformaldehyde (PFA) for 30 min at room temperature, and this procedure was repeated again. Cytospins were then immersed in 15% sucrose for 30 min and then rinsed in PBS to remove
sucrose. The cytospins were then dried overnight at 37° C incubator.
The slides were stored at 80° C pending analysis.
Differential Cell Count
A differential cell count was performed on unfixed cytospins of BAL cells using May-Grunwald Giemsa stain.
In Situ Hybridization
The cDNA fragment encoding FcRI (bp 25-936) was kindly provided by Dr. J.-P. Kinet (Molecular Allergy and Immunology Section, National Institute of Allergy and Infectious Diseases, Rockville, MD)
(19). This cDNA segment was inserted into the RNA expression vector (pGEM7) (Promega, Southampton, UK) and linearized to produce antisense and sense riboprobes. 35S-labeled riboprobes were prepared with Sp6 or T7RNA polymerase (Promega) to generate antisense
or sense probes, respectively. In situ hybridization (ISH) of cytospins
prepared from BAL cells were performed according to a protocol that
has been validated previously (16), with some modifications. In brief,
cytospins were made permeable by immersion in 0.3% Tritron × 100 in PBS for 10 min. After a brief washing in PBS, slides were further made permeable by exposure to proteinase K (Promega) solution (1 mg/ml in 20 mM TRIS-HCl and 1 mM EDTA at pH 7.2) for 20 min at
37° C, the activity of which was then terminated by immersion in 4%
paraformaldehyde/PBS for 5 min. To inhibit nonspecific binding of
35S-labeled probes, slides were treated with 10 mM iodoacetamide and
N-ethyl-malemide (Sigma) for 30 min at 37° C and then treated with
0.5% acetic anhydride and 0.1 M triethanolamine for 10 min before
air-drying. Slides were hybridized with 35S-labeled riboprobes (either
antisense or sense at 106 cpm per slide) at 55° C overnight. After hybridization, the slides were washed under high-stringency conditions
(65° C, 0.1 SSC). After dehydration, slides were immersed in K-5 emulsion (Ilford Ltd, Ilford, Essex, UK) and exposed for 2 weeks at 4° C. The autoradiographs were developed in developing solution (D-19;
Eastman, Kodak Co., Rochester, NY), fixed with Hypam (Ilford),
counterstained with hematoxylin and chromotrope 2R (BDH, Poole,
UK) for 30 min. For negative controls, slides were hybridized with a
sense probe or pretreated with RNase (Sigma) prior to hybridization
with the antisense probe.
Immunocytochemistry
A noncompetitive murine monoclonal antibody 22E7 (a kind gift
from Drs. R. Chizzonite and J. P. Kochan, Hoffman La Roche Inc., Nutley, NJ; concentration, 10 µg/ml) directed against the chain of
Fc RI was used for immunocytochemistry using the APAAP method (17). As a negative control, the primary antibody was replaced with
nonspecific mouse IgG.
Cells on cytospin slides were first treated with 1% hydrogen peroxide and 0.02% sodium azide in PBS to block endogenous peroxidase. Immunocytochemistry was then performed using a vector kit (Vector, Peterborough, UK) consisting of rabbit serum, noncompetitive murine monoclonal antibody 22E7 (10 µg/ml), biotinylated rabbit antimouse antibody, and avidin biotin complex. The reaction was developed in SG substrate (Vector). 22E7+ cells stained grey/black. Slides were then washed in water after immunocytochemistry and counterstained with chromotrope 2R (BDH) for 45 min. The slides were then dehydrated and mounted in DPX.
Quantification
Slides were counted blind in a random coded fashion using a BH2 microscope (Olympus Corp.) fitted with an eyepiece graticule. For in
situ hybridization studies, hybrids between FcRI chain mRNA and
cRNA probes were localized as dense collections of silver grains in
photographic emulsion overlying individual cells. Cells expressing
Fc RI chain-specific mRNA were quantified in terms of the number
of cells with overlying silver grains. For each subject (control and allergen challenged), at least 200 total BAL cells were counted. Chromotrope 2R+ cells (red color) were considered as eosinophils. For
immunocytochemistry, counts were performed at magnification ×200
and cells double-stained with FcRI+/chromotrope 2R+ were confirmed at magnification ×1,000 under oil immersion. For both techniques, random fields on slides were counted. Within-observer mean
coefficient of variation for cell counts was always less than 5%.
Statistical Analysis
Data were analyzed using a Microsoft Excel statistical package. Wilcoxon's matched-pairs signed-rank test was used for within-group comparisons. Between groups, the net increases in cell counts (allergen minus control) were compared using the Mann-Whitney U test. Correlation coefficients were obtained using Spearman's rank analysis; p values < 0.05 were considered significant.
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RESULTS |
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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Clinical
Relevant details of the patients and normal volunteers studied are shown in Table 1. The two groups were well matched for age and sex. All asthmatics had circulating Der p specific IgE, as demonstrated by positive RAST tests (mean, 38.5 IU/ml), whereas this was not detectable in the nonatopic control subjects (Table 1). The asthmatics also demonstrated airway hyperresponsiveness to inhaled histamine; mean value being 2.02 mg/ml (p < 0.05). Seven of the nine asthmatic subjects reacted to the instillation of Der p allergen by visible constriction of the challenged bronchus. This was accompanied by local wheezing determined by auscultation. At 24 h, slight mucosal swelling was visible in some of these patients, but the airway caliber appeared normal. No change in airway caliber was visible after saline control challenge. On the other hand, nonatopic normal subjects demonstrated no visible changes in airway caliber or hyperemia after both allergen and saline challenges.
BAL Differential Cell Counts
The absolute numbers of macrophages, lymphocytes, neutrophils, and eosinophils in lavaged bronchial segments after control saline and allergen challenge of atopic asthmatics and normal control subjects are shown in Figure 1. After segmental challenge with Der p, there was a significant increase in the absolute numbers of BAL eosinophils, median values of 0.15 × 106 (0 to 0.55 × 106) and 11.1 × 106 (0.5 to 46.5 × 106) cells (p = 0.007) for control and allergen, respectively (Figure 1). BAL lymphocytes and neutrophils also showed significant increases after allergen (Figure 1). On the other hand, no significant changes in BAL macrophages was observed after allergen provocation (Figure 1).
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BAL FcRI+ Cell Count
When compared with a control (diluent) challenge, in situ hybridization studies demonstrated a 6-fold increase in FcRI
mRNA+ cells after allergen; median values were 2 (0.7 to 7.2)
and 11.5 (0.6 to 65.0) × 106 cells for control and allergen, respectively (Figure 2A). Net increases in FcRI mRNA+ cells
correlated with the net increases in BAL eosinophils (r = 0.98, p = 0.0001). Similarly, the total numbers of FcRI chain protein-bearing cells also increased after allergen; median values
were 0 (0 to 0.30 × 106) and 3.1 × 106 (0.45 to 162.5 × 106)
cells (p = 0.007) (Figure 2B). Net increases in FcRI+ cells correlated with the net increases in BAL eosinophils (r = 0.72, p = 0.02). There was no significant change in FcRI+ cells in BAL after allergen in normal control subjects (Figure 2).
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Colocalization of FcRI mRNA and Protein
to BAL Eosinophils
In situ hybridization studies in nine asthmatics demonstrated
that only 4% of FcRI mRNA+ cells were colocalized to
chromotrope 2R+ eosinophils after saline (control) challenge
(Table 2). On the other hand, 85% of FcRI mRNA+ cells
colocalized to eosinophils after segmental allergen challenge
(Table 2 and Figure 3A and B). The eosinophil numbers were
very low in BAL after control challenge (1 to 2 per whole
fields counted), and 75% of them expressed Fc RI chain
mRNA. Segmental allergen challenge resulted in significant BAL eosinophilia (Figure 1), and 80% of these eosinophils
showed positive hybridization signals for FcRI mRNA.
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In order to confirm colocalization of FcRI chain protein
to eosinophils, colocalization studies with 22E7 and chromotrope 2R were performed in six asthmatic subjects who had
appreciable numbers of 22E7+ cells by single staining. These
studies revealed that 95% (93 to 96%) of Fc RI+ cells
stained with chromotrope 2R (Table 3 and Figure 3C and D).
We also examined the percentage of chromotrope 2R+ cells
in BAL that were immunostained with 22E7; 91% (26 to
100%) of 2R+ cells coexpressed the FcRI subunit. There
were no changes in FcRI+ cells, eosinophils, or other cell
populations in normal control subjects after allergen challenge (Figures 1 and 2).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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We have demonstrated increased numbers of FcRI mRNA
and protein-bearing cells in BAL of subjects with atopic
asthma after segmental allergen challenge. We confirmed that
the predominant FcRI+ cells (85 and 93%) in BAL after allergen exposure were eosinophils and 80 to 91% of the eosinophils expressed both mRNA and protein for FcRI+. The
fact that similar changes were not observed in the nonatopic
control subjects suggests that these changes are dependent
upon the presence of allergen-specific IgE and not upon some
nonspecific effect of locally instilled allergen.
Allergen-induced increases in BAL Fc RI+ cells were
observed in the asthmatics within the time frame of the late
phase bronchoconstrictor response to global allergen bronchial challenge, which is well known to be associated with a
dose-dependent influx of inflammatory cells, particularly eosinophils, lymphocytes, and neutrophils, into the bronchial lumen
18 to 24 h after allergen exposure (18, 20, 21). The advantage
of the segmental challenge model is that it allows simultaneous challenge with allergen and diluent in remote bronchial
segments, thus ensuring that each subject acts as his or her
own control. The disadvantage is that global bronchoconstrictor responses cannot be measured. Nevertheless, seven of the
nine atopic subjects in our study clearly demonstrated an immediate segmental bronchial response 5 to 10 min after allergen challenge, and this observation coupled with the characteristic inflammatory cell influx 24 h later provide compelling
evidence that the observed allergen-induced increases in
FcRI+ cells in the asthmatics occurred within the context of
a late phase inflammatory response to allergen challenge.
In this study we took mRNA and protein expression of the
chain of the high affinity receptor for IgE (FcRI) as an indicator of their potential to be activated by IgE-mediated mechanisms. Because cytospins were used in this study some immunostaining may reflect intracellular rather than membrane
staining. The biologic importance of FcRI in mediating IgE-dependent immune reactions has been demonstrated in a
number of different studies (5, 14, 22). It has been speculated that eosinophils may also be involved in antigen presentation in allergic diseases via IgE linked to FcRI (28). FcRI
has also been implicated in IgE-dependent schistosomal killing by eosinophils (14).
Our data show that a median of 80 to 91% of eosinophils
recruited to the bronchial lumen of atopic asthmatics 24 h after
local allergen challenge expressed the chain of FcRI, although
there was some variability in this figure. Furthermore, eosinophils comprised a median of 85 to 95% of the total FcRI+
cells so recruited (Tables 2 and 3). Our results are consistent
with those observed by Barata and colleagues (16) in the skin
after allergen challenge. These findings contrast strikingly
with the distribution of FcRI chain expression on cells
within the bronchial mucosa and peripheral blood of stable,
atopic asthmatics at "baseline" (i.e., in the absence of allergen
challenge). We found some FcRI mRNA expression after
control challenge in both asthmatics and normal subjects, but
no significant protein expression was seen (Figure 2). This dichotomy might be due to the difference in sensitivity of the
two methods employed. However, only a few eosinophils were present after control challenge expressing Fc RI mRNA,
and only 4% of FcRI mRNA+ cells were eosinophils at
"baseline" (control challenge). Consistent with this, three recent studies on such patients have suggested that, in both the
bronchial mucosa and the peripheral blood, mast cells/basophils and monocytes/macrophages constituted the majority of
FcRI+ cells, whereas eosinophils made up only a small percentage (17, 29, 30). The remainder of the FcRI+ cells recovered from the bronchial lumen of the atopic asthmatics after allergen challenge in the present study were presumably
other cells (monocyte/macrophages, mast cells/basophils and
dendritic cells) known to express FcRI constitutively (12, 13, 17, 29, 30). Our data do not permit accurate quantification of the distribution of FcRI+ expression on these cells. Because the numbers of FcRI+ cells and eosinophils in the
bronchial lumen of the atopic asthmatics after control challenge were in general very low, our data considered with the
data referred to the above concerning FcRI expression in
the blood and bronchial mucosa of these patients suggest a
process whereby eosinophils expressing both mRNA and protein for FcRI are preferentially recruited to the bronchial
lumen of these patients. The mechanism of this process remains to be defined, but it might include synthesis and upregulation of FcRI expression on eosinophils in transit from the
peripheral blood to the bronchial lumen after interaction with
cytokines such as IL-5, IL-3, or GM-CSF (31), selective recruitment of FcRI-expressing eosinophils from the blood or bronchial mucosa, or both. Again, this process would appear
to be IgE-dependent since it was not observed in the nonatopic control subjects in the present study after allergen challenge under identical conditions.
There are early indications that FcRI expression on eosinophils may play an important role in mediating eosinophil
function in inflammatory processes. In peripheral blood monocytes, allergen-specific IgE bound to surface FcRI receptors
has been shown to enhance allergen presentation to T cells,
and it has been speculated that eosinophils may also present
antigen in this way (26). Gounni and colleagues (14) provided
the first evidence that cross-linking of Fc RI receptors on
eosinophils obtained from patients with hypereosinophilic syndrome resulted in eosinophilic degranulation and participated
in eosinophil-mediated cytotoxicity against Schistosoma mansoni. Release of cationic proteins such as major basic protein (MBP), eosinophil cationic protein (ECP), eosinophil-derived
neurotoxin (EDN), and eosinophil peroxidase (EPO) are believed to mediate, at least in part, the bronchial epithelial
damage characteristic of asthma (31).
We therefore propose that, in vivo, allergen exposure in
sensitized asthmatics not only upregulates eosinophilopoesis
and eosinophil recruitment to the site of allergen exposure but
also upregulates expression of FcRI mRNA and protein by
these cells. Our study indicates that, in contrast to mast cells,
macrophages, and dendritic cells, which constitutively express
FcRI, eosinophils may be the predominant cells in BAL expressing FcRI after endobronchial allergen exposure. This
raises the possibility that FcRI-expressing eosinophils may
therefore participate in IgE-mediated allergic inflammatory
responses. Further studies should focus on the regulation and
functional significance of FcRI expression by eosinophils and
their IgE-dependent activation.
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Footnotes |
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Correspondence and requests for reprints should be addressed to Dr. K. Rajakulasingam, Department of Respiratory Medicine, Homerton Hospital, Homerton Row, London E9 6SR, UK.
(Received in original form August 26, 1997 and in revised form February 5, 1998).
Acknowledgments: Supported by a National Asthma Campaign (UK) Project Grant.
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References |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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