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ABSTRACT |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Measures of airway inflammation are increasingly being used as outcome measures in asthma intervention studies. Meaningful interpretation of observed changes in bronchial mucosal cell numbers should depend, in part, on the reproducibility of repeat measures over time. We wanted to investigate the reproducibility of immunopathologic and physiologic parameters after short and long
measurement intervals. We therefore performed spirometry, bronchial provocation challenge, and
fiberoptic bronchoscopy with endobronchial biopsy (always right upper lobe second-generation
bronchus) at baseline, after 2 wk, and again after 8 wk on nine subjects with stable atopic asthma
(receiving inhaled placebo and 
-agonist therapy only). Numbers of T cells, memory T cells
(CD45Ro+), macrophages (CD68+), and eosinophils (EG1+ and EG2+) on immunohistochemical
stains of bronchial biopsies were quantified by computerized image analysis. Intraclass correlation
coefficients (ICCs) of reproducibility were calculated for repeat measures of each parameter and a
high ICC (greater than 0.6) was interpreted as "highly reproducible." Repeat measures of FEV1,
FEF25-75%, and PC20 were highly reproducible after short (2-wk) and long (8-wk) intervals. Only repeat measures of EG2+ had an ICC greater than 0.6 after 8 wk. Repeat measures of CD45Ro+, EG2+,
and T cell numbers (but not CD68+ and EG1+ cells) are highly reproducible and reliable parameters
of asthmatic airway inflammation after a 2 wk interval. Faul JL, Demers EA, Burke CM, Poulter
LW. The reproducibility of repeat measures of airway inflammation in stable atopic asthma.
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Research on endobronchial biopsies (pre- and post-therapy) has been widely used to assess the effects of provocation and antiasthma therapy on airway inflammation (1). Measured changes in numbers of inflammatory cells between biopsies (obtained after various time intervals) have generally been interpreted as pro- or antiinflammatory effects of an intervention. However, these changes may be due to other factors, including measurement error (attributable to the measurement instrument) and/or the natural variability of airway inflammation over time. In the interpretation and design of intervention biopsy studies, it is worthwhile to consider the changes in biopsy parameters that may occur owing to the variability of airway inflammation over time before ascribing observed changes to an intervention. In the setting of asthma research, it is particularly important to distinguish between changes that can be properly attributed to an intervention and those that may be due to natural variability, because biologic variability is the defining characteristic of bronchial asthma (5). Type 2 errors might readily occur in asthma intervention studies that employ unreliable biomarkers such as asthma outcome measures, because changes in a measure may be falsely explained by an effect of an intervention, rather than by biologic variability (6). We therefore wanted to assess the reproducibility of repeat measures of bronchial mucosal inflammatory cell numbers in subjects with stable asthma after short (2-wk) and long (8-wk) sample intervals.
Airway inflammation in clinically stable asthma has been shown to exhibit considerable biologic variability (7). Few data exist, however, on the effect that the duration of biopsy interval has on the reproducibility of repeat measures of inflammatory cell numbers. Such data are fundamental to the interpretation of biopsy studies, because the usefulness of employing airway inflammatory cell numbers as markers of disease activity depends, at least in part, on their reproducibility over time. In a previous study of the immunopathology of asthma we have demonstrated that, at a single time point, there is little variability in repeat measures of inflammatory cell numbers within the same tissue section (11). In addition, the variability in repeat measures of inflammatory cell numbers in different sections of the same biopsy was consistently less than 10% (11). Greater intrasubject variations occur between measures from biopsies from different areas of lung (e.g., proximal and distal airways) (11). Other workers, using similar methods, have also demonstrated that the variability of repeat measures, both within a single tissue section and within different sections of a single biopsy, is small (9, 10). However, the variability of repeat measures of inflammatory cell numbers in different biopsies consistently outweighs within-biopsy variability (10). To date, the effect of the length of sampling interval on the reproducibility of measures of airway inflammation is unknown. We therefore designed the current study of patients with stable asthma in order to compare the effects of short and long interval duration on the reproducibility (and by implication reliability) of repeat measures of airway inflammation in serial bronchial biopsies.
The intraclass correlation coefficient (ICC) is a dimensionless statistic that describes the reproducibility of repeat measures in the same population (12). The value of ICC is bounded by 0 and 1. An ICC value of 1 for repeat measures indicates perfect reproducibility, whereas a value of 0 is interpreted as reproducibility that is no better or worse than expected by chance. In a stable population, repeat measures with an ICC value in excess of 0.6 are thought to be clinically useful. Repeat measures with an ICC value of less than 0.6 are probably not. In this article the ICC is employed to quantify between-biopsy reproducibility of repeat measures in the same subjects after short and long sample intervals. By quantifying the reproducibility of physiologic and inflammatory cell measures over time, this study is a unique description of the variability of airway inflammation in stable asthma.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Subjects
Nine subjects with atopic asthma subjects (American Thoracic Society criteria [5] for asthma) were recruited (age, 18-40 yr; seven males) (see Table 1). None had suffered an exacerbation of asthma or taken corticosteroid therapy during the previous 3 mo. Baseline FEV1 for all subjects was greater than 40% predicted and all subjects showed at least a 250-ml (and 12.5%) increase in FEV1 after inhaled salbutamol. All subjects demonstrated bronchial hyperreactivity, evidenced by a histamine PC20 (provocative concentraton of an agonist causing a 20% fall in FEV1) of < 8 mg/ml, within 4 wk of entry (13). Subjects were excluded if they were pregnant or lactating, had a psychiatric illness, or other concurrent clinical condition. Supplementary oral or inhaled corticosteroids, theophyllines, cromolyns, and leukotriene antagonists were not allowed. Rescue inhalers were confined to salbutamol by metered dose inhaler. The Ethics Committee of James Connolly Memorial Hospital (Dublin, Ireland) approved the study protocol. Full written informed consent was obtained from each subject. The nature of the study demanded that great care be taken to provide an easily accessible and prompt medical backup for the subjects enrolled. A team of senior clinicians was on call on a 24-h/7-d basis to provide continuous medical backup. Investigators were available at all times for unscheduled visits to hospital and to ensure early withdrawals from the study in the event of deteriorating asthma or intercurrent illness.
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Study Design
Each subject underwent fiberoptic bronchoscopy and endobronchial biopsy on three occasions: at baseline, after 2 wk, and after 8 wk (14). During a 1-wk run-in period and throughout the study period, subjects used a placebo inhaler (four puffs twice daily by metered dose inhaler attached to an aerosol chamber [Volumatic spacer; Allen & Hanburys, Greenford, UK]) and recorded peak expiratory flow rates (PEFRs) (morning and evening) using a mini-Wright peak flow meter. Subjects were instructed to contact the principal investigator (and were withdrawn) if PEFRs declined by more than 20% compared with the baseline mean PEFR determined during week 1.
Bronchodilator medication and caffeine-containing drinks were withheld for at least 12 h before each study visit and subjects always attended the laboratory at 9:00 A.M. Physical examination and routine blood and urine tests were performed before each bronchoscopy. Bronchodilator responses were always studied 4 h before bronchoscopy: FEV1 was measured before and 20 min after salbutamol (200 µg) was administered via a Volumatic spacer device. The bronchodilator response was expressed as the percentage change in FEV1 (postbronchodilator) from baseline.
The use of bronchodilator medication and adverse events were checked and recorded at each clinic visit. FVC and FEV1, bronchodilator response, FEV1/FVC, and FEF25-75% were recorded using a Gould 2400 computerized spirometer. One day before to each bronchoscopy, histamine bronchial provocation challenges were performed according to a standardized technique (13). A complete dose- response curve for inhaled histamine was recorded, using doubling concentrations starting with 0.03 mg/ml and ending with 16 mg/ml of histamine dissolved in normal saline. During histamine challenges FEV1 was measured 30 and 90 s after each dose. The test was terminated if FEV1 decreased by more than 20% from the postsaline value or if a concentration of 16 mg/ml was reached. Histamine PC20 was determined by linear interpolation of the concentration FEV1 response curve. Subjects were not allowed salbutamol for 12 h before bronchial challenge. Allergy tests were performed at the screening visit. Subjects were considered atopic if they gave a history of bronchospasm after allergen exposure and exhibited a positive skin prick test (> 3-mm-diameter wheal reaction) to at least one of a panel of common allergens (house dust mite, grass pollen, cat, dog, and birch pollen).
Fiberoptic Bronchoscopy
Each subject underwent flexible fiberoptic bronchoscopy (Olympus,
Norwood, MA) on three occasions (Days 0, 14, and 56) (14). Topical
anesthesia was obtained by administration of 1% lignocaine to the vocal cords. Subjects were sedated with intravenous propofol (15) and
continuous oxygen was administered by nasal cannulae. Oxygen saturation and electrocardiogram (ECG) were monitored throughout the
procedure. Up to three endobronchial biopsies were taken through the bronchoscope with spiked cup forceps, always from the second-generation right upper lobe bronchus. Biopsies were immediately
placed on sterile phosphate-buffered saline (PBS)-moistened gauze,
embedded in O.C.T. medium (Miles, Elkhart, IN) and snap frozen in
cooled (in a liquid nitrogen bath) isopentane. The samples were
stored in liquid nitrogen until further analysis. Cryostat sections (6 µm
thick) of the endobronchial biopsies were cut at 
25° C, air dried for
1 h, then fixed in chloroform-acetone (1:1, vol/vol), wrapped in cling
film, and stored at 20° C until use. Representative sections of all
samples were stained with 0.1% toluidine blue to reveal appearance
and tissue integrity. Immunohistological techniques were employed to
identify cell types. The indirect immunoperoxidase technique (1, 2,
11) was used to identify T cells (using a cocktail of monoclonal antibodies (MAbs) to CD2, CD3, CD7, and CD8), memory T cells (MAb
to CD45Ro), macrophage-monocytes (MAb to CD68), total eosinophils (MAb to EG1), and "activated" eosinophils (MAb to EG2).
Quantification of Immunohistology
All bronchial biopsies were stored in liquid nitrogen and subsequently processed in random time order, in order to avoid any measurement error being attributed to a technical or learning effect. An investigator with no knowledge of the identity, therapy, or timing of biopsies (L.W.P.) quantified the numbers of cells. The presence, distribution, and number of each cell type were assessed using a "Solitaire" (Seescan, Cambridge, UK) computerized image analysis system. Three areas of epithelium and subepithelial connective tissue to a depth of 10 to 12 cells were measured in each section. Total areas of 12 × 104 µm were quantified on duplicate sections for each cell type in samples for each biopsy. Areas of each high-power field measured were determined with the image analyzer by drawing frames around the area to be quantified. These frames were designed to avoid damaged areas and areas of muscle. Numbers of positive cells within framed areas were point counted and all results were then reduced to cells per unit area by dividing the number of cells documented in each field by the area of section in square micrometers calculated by the computer, as previously described (11). Average numbers of cells per unit area (for three areas) were calculated for each cell type at each time point.
Statistics
To quantify the repeatability of measures on the same group of subjects, the intraclass coefficient (ICC) was employed (12). The ICC
represents an estimate of the average correlation between all possible
ordering of pairs of measures. For each sample interval (two sets of
data; e.g., data at 2 wk compared with baseline) the total sum of
squares (SST) and the sum of squares between subjects (SSB) were derived with a one-way analysis of variance table. The ICC was calculated as follows: ICC = [(2 × SSB) SST]/SST. ICCs were calculated
for both immunopathologic and physiologic parameters. To determine if any significant within-group changes occurred during the
course of the study, the significance of within-group changes (after 2 and 8 wk) was estimated using two-way ANOVA.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The subjects in this study formed part of a large biopsy controlled trial of inhaled corticosteroids in asthma (1). Nine subjects with stable atopic asthma were randomized to receive placebo. All subjects completed the protocol, each with three endobronchial biopsies. There were no dropouts. The results of computerized spirometry, histamine provocation challenges, and bronchial mucosal cell numbers are contained in Table 2. These data confirm airway physiology consistent with mild asthma. Taken as a group, no significant change in airway physiology or inflammation was observed after 2 or 8 wk of therapy with inhaled placebo (two-way ANOVA).
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The intraclass correlation coefficients for repeat physiologic measures are presented in Figure 1. Postbronchodilator FEV1 was the most reproducible index of spirometry: the repeat measures ICC was 0.95 at 2 wk, compared with a 2-wk ICC of 0.89 for FEF25-75%, and ICC of 0.7 for bronchodilator response. After 8 wk the repeat measures ICCs for these indices were 0.75, 0.68, and 0.56, respectively. Repeat measures of PC20 were highly reproducible at both 2-wk (ICC equal to 0.71) and 8-wk (ICC equal to 0.88) intervals.
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Intraclass correlation coefficients for repeat measures of immunologic indices are presented in Figure 2. Repeat measures of T cell (ICC equal to 0.81), CD45Ro+ cell (ICC equal to 0.70), and EG2+ cell (ICC equal to 0.67) numbers appeared highly reproducible after a 2-wk sample interval. After 8 wk, the ICCs for repeat measures of these parameters were equal to 0.41, 0.51, and 0.73, respectively. Only repeat measures of EG2+ cell numbers remained highly reproducible (ICC equal to 0.73) after an 8-wk interval. Repeat measures of CD68+ and EG1+ cells were less reproducible after both a 2-wk interval (ICC equal to 0.23 and 0.40, respectively) and after an 8-wk interval (ICC equal to 0.07 and 0.26, respectively) (Figure 2).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Intervention biopsy studies of the effects of antiasthma therapy
on airway inflammation have provided valuable information about disease mechanisms in asthma (1, 3). The design of biopsy studies in asthma is an area of considerable research because antiinflammatory agents and modes of their administration are currently being developed and investigated by such
methodology (1, 16). However, the design of biopsy studies in
subjects with asthma is fraught with logistic, technical, and
ethical problems (17). The situation is further complicated by
uncertainty regarding the optimal time interval between biopsies. Until now, no clear data have existed on the optimal duration of bronchial biopsy studies and time intervals between
biopsies are chosen on an arbitrary basis (sampling intervals
of 2, 4, 6, 8, and 12 wk have been employed). The current
study demonstrates that the reproducibility of repeat measures
of airway inflammation in stable asthma (on inhaled -agonist and inhaled placebo therapy only) is significantly greater
after a 2-wk interval rather than after a 2-mo interval. Repeat
measures of most inflammatory cells are less reproducible
and are probably clinically unreliable after an 8-wk biopsy
interval. The current data suggest that, in studies of asthmatic
airway inflammation, shorter intervals (of 2 wk or less) between sampling may minimize type 2 errors due to the variability of inflammatory cell counts. In addition, this study has
determined that repeat measures of some parameters, such as
T cells, memory T cells (CD45Ro+) and EG2+ cells are highly
reproducible (after a 2-wk interval). These parameters should
provide the most reliable information about the severity of
airway inflammation in stable asthma. Notably, repeat measures of airway EG2+ cells appear particularly reproducible
(18) after short and long sampling intervals. This biopsy study
demonstrates that repeat measures of most airway inflammatory cell numbers (the "gold standard" markers of airway inflammation) are unreliable after an 8-wk sampling interval.
The implication is that surrogate markers of airway inflammation (serum and sputum markers) need to be carefully validated in terms of reliability, especially over long measurement intervals.
In contrast to previous studies of the variability of inflammatory parameters in asthma (9, 10), this study has examined endobronchial biopsies at three time points. We demonstrate that repeat measures of some airway inflammatory cell numbers are highly reproducible after 2 wk, and are likely to be reliable indices of airway inflammation over this period. More importantly, the data demonstrate, for the first time, that repeat measures of most parameters of airway inflammation become less reproducible with length of biopsy interval. The reproducibility of repeat measures of airway inflammatory cells after 2 wk compared with after 2 mo demonstrates that most repeat measures are less repeatable after longer biopsy intervals and therefore are probably not clinically useful (12). The implication is that intervention studies with longer biopsy intervals could lead to type 2 errors because observed differences in some inflammatory cell numbers might be falsely attributed to the effect of an intervention rather than to biologic variability. One can hypothesize that in order to estimate the correct interval between biopsies, there would appear to be a trade-off between longer biopsy intervals, which allow greater time for the biologic effect of an intervention, and shorter sampling intervals, which help to minimize the effect of biologic variability. Such factors should be carefully considered when designing or assessing studies that use biopsies as outcome measures.
This study analyzes immunopathologic data obtained from
serial biopsies of subjects with clinically stable asthma and
who received inhaled -agonist and inhaled placebo therapy.
The data demonstrate that repeat measures of some lymphocyte (T cells and CD45Ro+ [memory] T cells) and eosinophil
(EG2+) subsets are highly reproducible and may provide the
most useful, reliable information when the effects of therapy,
allergen, or infection on the inflammatory cell profile of the
asthmatic airway are studied. Repeat measures of other inflammatory cells (CD68+ cells and EG1+ cells) were less reproducible in the setting of clinically stable asthma and are
probably unreliable indices. Given the variability of repeat
measures of airway inflammation in this study of subjects with
mild asthma, one can only speculate that the variability of inflammation over time is far greater in severe or clinically unstable asthma.
Another important issue in the interpretation of bronchial biopsy studies is the potential effect of tissue injury, occurring during the act of fiberoptic bronchoscopy and endobronchial biopsy, on future measures of airway inflammation. In theory, the healing process that occurs after biopsy might significantly alter measures of inflammatory cells in the bronchial mucosa at a subsequent biopsy. These effects might be important if the same general anatomic site is being biopsied on more than one occasion. The results of this study are reassuring in this regard. Our results demonstrate that repeat measures of inflammatory cell numbers are more reproducible after a 2-wk interval than after an 8-wk interval. This suggests that the variability of airway inflammation over time probably outweighs the acute effects of bronchoscopic biopsy. We cannot exclude the possibility that the act of bronchoscopic biopsy might lead to acute changes in CD68+ and EG1+ cells, thus accounting for their poor reproducibility on repeat biopsy 2 wk later. We do not know how much time is needed to recover from bronchoscopic biopsy, but the current study suggests that recovery from endobronchial biopsy almost certainly occurs within 2 wk.
Since the introduction of fiberoptic bronchoscopy, there
has been considerable interest in the use of repeat bronchial
biopsy studies to assess disease mechanisms in asthma. However, in contrast to the wealth of data that supports the use of
highly reproducible physiologic measures (e.g., FEV1, PC20) as
reliable indices of airflow limitation and disease severity (20,
21), few data exist on the reliability of repeat measures of airway inflammation (17). This article describes the reproducibility of repeat measures of airway inflammatory cell numbers in
a group of patients with stable asthma and who are not receiving antiinflammatory therapy (inhaled placebo and -agonist
therapy only). The lack of significant (within-group) changes
in measures of bronchodilator responses, and spirometry confirms that these subjects had stable asthma throughout the
study (1). Measures of peak flows and peak flow variability
were stable throughout and no significant clinical exacerbation was observed or treated during the course of the study.
Our results are consistent with others who have demonstrated that repeat measures of some physiologic indices (e.g., FEV1) are highly reproducible (20). Oldham and Cole, for instance, have demonstrated an ICC of 0.99 for repeat FEV1 measures
taken on the same day and an ICC of 0.88 for repeat measures
after a 2-wk interval (22). The data in this study are in agreement with conventional wisdom: repeat measures of FEV1 and
PC20 are highly reproducible and the current data support
their use as reliable parameters of asthmatic physiology (20, 21).
To assess the reproducibility of repeat measures of airway inflammation in asthma (and, in contrast to previous studies, of the variability of airway inflammation in asthma [9, 10]), we examined serial bronchial biopsies from subjects with mild/ moderate asthma who received no antiinflammatory therapy (i.e., those who took placebo inhalers) for the duration of the study. This study was designed for two reasons to examine multiple bronchial biopsies obtained from patients with asthma and not taking inhaled steroids. First, it is now well established that corticosteroids have profound effects on airway inflammation in asthma (19). Steroid therapy has previously been shown to have significant effects on airway physiology and numbers of inflammatory cells in the bronchial mucosa in asthma (1, 16, 19); therefore changes in repeat measures of these parameters in subjects receiving corticosteroid therapy could be attributable to the effects of therapy. Second, corticosteroid therapy is likely not only to downregulate airway inflammation but also to dampen its biologic variability (just as it appears to dampen the variability of airway physiology). For both these reasons care was taken to ensure that only patients with clinically stable asthma and not receiving corticosteroid therapy (inhaled placebo therapy only) were examined. Evidence that the participants had clinically stable asthma is revealed by the lack of spirometric or peak flow deterioration during the study. Moreover, there was no significant (within-group) change in airway physiology or immunopathology after 2 or 8 wk, as assessed by two-way ANOVA (Table 2). Because the subjects in this study did not receive antiinflammatory therapy (which might downregulate inflammatory cell numbers) the current data provide a unique description of the natural variability of airway inflammation in clinically stable asthma.
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Footnotes |
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Correspondence and requests for reprints should be addressed to Professor Leonard W. Poulter, Department of Clinical Immunology, Royal Free Hospital School of Medicine, Pond St., London NW3 2PE, UK.
(Received in original form December 4, 1998 and in revised form April 6, 1999).
Acknowledgments: The authors are grateful to Shelley Poulter, Department of Immunology, Royal Free Hospital School of Medicine, London, for technical assistance.
Supported by Glaxo/Wellcome Research & Development UK, Ltd.
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References |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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 S. O'Sullivan, L. Cormican, M. Murphy, L. W. Poulter, and C. M. Burke Effects of Varying Doses of Fluticasone Propionate on the Physiology and Bronchial Wall Immunopathology in Mild-to-Moderate Asthma Chest, December 1, 2002; 122(6): 1966 - 1972. [Abstract] [Full Text] [PDF]
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J. L. Faul, E. A. Demers, C. M. Burke, and L. W. Poulter Alterations in Airway Inflammation and Lung Function During Corticosteroid Therapy for Atopic Asthma* Chest, May 1, 2002; 121(5): 1414 - 1420. [Abstract] [Full Text] [PDF]
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B. D. Stone, T. Elias-Todd, J. Parrino, C. Ward, E. H. Walters, J. L. Faul, C. M. Burke, and L. W. Poulter EG-1 POSITIVE EOSINOPHILS IN ASTHMA Am. J. Respir. Crit. Care Med., July 1, 2001; 164(1): 171a - 172. [Full Text] [PDF]
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W. J. CALHOUN, K. L. HINTON, and J. J. KRATZENBERG The Effect of Salmeterol on Markers of Airway Inflammation Following Segmental Allergen Challenge Am. J. Respir. Crit. Care Med., March 15, 2001; 163(4): 881 - 886. [Abstract] [Full Text]
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