Lung accumulations of eosinophil granulocytes after exposure to cornstarch glove powder

doi:10.1183/09031936.03.00024103

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Lung accumulations of eosinophil granulocytes after exposure to cornstarch glove powder

J. Grunewald¹, A. Eklund¹, K. Katchar¹, A. Moshfegh², C. Lidén³, L. Lundgren⁴, L. Skare³ and G. Tornling¹^,5

Divisions of ¹ Respiratory Medicine, ² Clinical Immunology and Allergy, Dept of Medicine, Karolinska Hospital and Institutet, ³ Occupational and Environmental Dermatology, Dept of Medicine, Karolinska Institutet and Stockholm County Council, ⁴ Workplace Air, National Institute for Working Life and ITM, Stockholm University, Stockholm, and ⁵ Clinical Science, Astra Zeneca, Lund, Sweden

CORRESPONDENCE: J. Grunewald, Dept of Medicine, Lung Research Laboratory L2:01, Karolinska Hospital, S-171 76 Stockholm, Sweden. Fax: 46 851775451. E-mail: johan.grunewald@medks.ki.se

Keywords: bronchoalveolar lavage, cornstarch glove powder, eosinophil granulocytes

Received: March 25, 2002
Accepted November 29, 2002

This study was supported by the Swedish Council for Work Life Research (RALF), the Swedish Heart-Lung Foundation, the King Oscar II Jubilee Foundation, the Swedish Foundation for Health Care Sciences and Allergy Research and Karolinska Institutet.

Abstract

TOP
Abstract
Material and methods
Results
Discussion
Acknowledgements
References

Starch is a main component of wheat flour, which, besides beingan occupational allergen can also induce irritative symptomsin the airways. A purified starch product (cornstarch glovepowder) was used to investigate whether starch alone could induceairway inflammation. The aim of the study was to investigatea role for starch in wheat flour-induced airway inflammation.

Ten healthy individuals were exposed to cornstarch glove powderin a whole-body exposure chamber. Bronchoscopy with bronchoalveolarlavage (BAL) was performed 2–3 weeks before and 1 dayafter exposure, and the BAL cells were counted differentially.In addition, the expression of activation, adhesion and subsetmarkers on alveolar macrophages and BAL T-cells were investigatedusing flow cytometry.

A three-fold increase in BAL cell concentrations was found,with a selective accumulation and activation of eosinophilicgranulocytes, as well as an influx of nonactivated monocytesand polyclonal CD4+ T-cells into the airways.

The results show that inhalation of cornstarch glove powderleads to the development of a subclinical inflammation in theairways, with an accumulation of eosinophilic granulocytes.The authors suggest that such exposure may be an interestingmodel for studying factors contributing to lung accumulationsof eosinophil granulocytes in humans.

Wheat flour is an occupational allergen related to an increasedrisk of developing chronic airway symptoms (baker's asthma)1. The authors have previously registered signs of airway inflammationin healthy individuals exposed to wheat flour (unpublished data)in a whole-body exposure chamber 2. It is not known to whatextent wheat flour components other than proteins, such as starch,may contribute to the induction of airway inflammation. Closeto one-third of bakers with asthma and/or rhinitis did not haveimmunoglobulin (Ig)E antibodies specific to any of the bakeryallergens 1. Following exposure to cornstarch particles fromstarch-powdered gloves, used in surgical procedures, a granulomatousinflammation of peritoneal surfaces was described 3, 4. Starchalso functions as a carrier of latex particles, for example,and starch-powdered gloves could induce an IgE-mediated asthmaticresponse in latex-sensitised individuals 5, 6.

The aim of this study was to investigate whether starch alonecould induce alterations in inflammatory parameters in the airways.Ten healthy individuals were exposed to an airborne total dustconcentration of 5.9 mg·m^–3 (median) cornstarchglove powder for 1 h, using a whole-body exposure chamber2. Cells were obtained from the lungs through bronchoscopy withbronchoalveolar lavage (BAL) 2–3 weeks before and 1 dayafter exposure. Differential counts were performed on BAL cells,and flow cytometry analysis of the expression of adhesion, activationand subset markers on alveolar macrophages (AM) and T-cellswas carried out. The results indicate that cornstarch glovepowder induces an accumulation of activated eosinophils intothe alveoli, together with an influx of AM and T-cells, butwithout clinical signs of airway symptoms.

Material and methods

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Abstract
Material and methods
Results
Discussion
Acknowledgements
References

Subjects
Ten healthy individuals (five males, five females, aged 18–49 yrs(median 26 yrs)) were included in the study. None of theseindividuals had a history of atopy, and they all had normalserum IgE values (<120 U·L^–1) as well asnormal radioallergosorbent tests specific for corn starch. Allindividuals were nonsmokers and all had normal chest radiographsand were without signs of any respiratory infection 1 monthbefore and at the time of the study. Informed consent was obtainedand the local ethics committee approved the study.

Study design
Each individual was exposed to cornstarch glove powder (Absorbo^TM;National Starch and Chemical Corporation, Bridgewater, NJ, USA)for 1 h in the whole-body exposure chamber. Cornstarchglove powder is an absorbable powder prepared by processingcornstarch in accordance with the requirements of the US PharmacopeiaMonographs on Absorbable Dusting Powder as well as the BritishPharmacopeia Monographs on Steralisable Maize Starch. It wastested by low-temperature ashing and found to contain 96–98%organic materials, i.e. corn starch, and magnesium oxide (MgO).No endotoxins could be detected in the powder (Multi-test LimulusAmebocyte Lysate; BioWhittaker, Walkersville, MD, USA). Totaldust was sampled in 37 mm open-faced cassettes on membranefilters made of mixed esters of cellulose (pore-size 0.8 µm)at flow rate 2 L·min^–1. Respirable dust (smallairborne particles that can penetrate into the gas-exchangeregions of the human lung) was sampled with cyclones (CasellaSIMPEDS; Casella London Ltd, London, UK) on membrane filtersmade of mixed esters of cellulose (pore-size 8 µm)at 1.9 L·min^–1.

Peripheral blood and BAL samples were obtained 2–3 weeksbefore and 1 day after the dust exposure. In addition, a third(follow-up) bronchoscopy with BAL was performed 7–8 monthsafter the cornstarch glove powder exposure in the four individuals(subject nos 4, 6, 7 and 9) exhibiting the most pronounced accumulationof lung eosinophils.

Bronchoalveolar lavage and handling of cells
Bronchoscopy with BAL was performed as described previously7. Briefly, BAL fluid was retrieved by instilling five aliquotsof 50 mL sterile phoshate-buffered saline (PBS) solutionat 37°C in a middle lobe bronchus. After each instillation,the fluid was gently aspirated and collected in a siliconisedbottle kept on ice. Mean recovery was 75% (interquartile range69–82%) at the first and 72% (68–82%) at the secondBAL.

The BAL fluid was strained through a double layer of Dacronnets (Millipore, Bedford, Ireland) centrifuged at 400xg for10 min at 4°C and the cells were resuspended in RoswellPark Memorial Institute (RPMI) 1640 (Sigma Aldrich Co., St Louis,MO, USA). The BAL fluid cells were counted in a Bürkerchamber and cell viability was determined by Trypan blue exclusionas 93% (91–95%) at the first and 92% (90–94%) atthe second BAL. For differential cell counts, cytospins wereprepared by cytocentrifugation at 20xg for 3 min and stainedin May-Grünwald Giemsa. Peripheral blood lymphocytes wereseparated from heparinised peripheral blood by Ficoll-Hypaque(Amersham Pharmacia Biotech, Uppsala, Sweden) gradient centrifugation,washed twice and diluted in RPMI 1640.

Immunostaining and flow cytometry
Immunolabelling of alveolar macrophages was performed usingprimary nonconjugated monoclonal antibodies (Mab) specific forCD11b (CR-3), CD14 (lipopolysaccharide receptor), CD16 (Fc ${gamma}$ RIII),CD54 (intercellular adhesion molecule-1), CD86 (costimulatorymarker) and human leukocyte antigen (HLA) class I and II (activationmarkers), followed by a secondary Rhodophyta phycoerythrin (RPE)-conjugatedMab. Antibodies with isotype-matched controls were obtainedfrom DAKO (Glostrup, Denmark).

BAL and peripheral blood CD4+ and CD8+ T-lymphocytes were detectedusing RPE-Cy5 conjugated CD4, RPE-conjugated CD8 and fluoresceinisothiocyanate (FITC)-conjugated CD3 Mab (DAKO). Triple stainingof cells was performed to determine the expression of activationmarkers by CD4+ and CD8+ cells, respectively, and to assessthe percentage of CD3+ cells that expressed CD4 and CD8. FITC-labelledMab specific for CD25 (interleukin-2R, early activation; DAKO),CD26 (activation, costimulation; Pharmingen, La Jolla, CA, USA),CD28 (costimulation; Coulter Immunotech, Marseille, France),CD57 (subset marker; Becton Dickinson, San José, CA,USA), CD69 (very early activation; Becton Dickinson) and HLA-DR(late activation; Becton Dickinson) were used. After antiserumincubations and washings, cells were fixed in PBS with 1% formaldehyde.The samples were analysed in a flow cytometer (FACSort; BectonDickinson). The cell populations were identified and gated byforward- and side-light scattering properties. For AMs, thequantitative level of expression of each antigen (mean fluorescenceintensity) was determined after subtraction of the backgroundfluorescence intensity levels. For lymphocytes, the percentagesof positively labelled cells in the CD4+ and CD8+ subsets weredetermined, respectively. Isotype-matched negative control antibodiesalways stained <1% of CD4+ and CD8+ lymphocytes.

Bronchoalveolar lavage fluid analyses
BAL fluid eosinophil cationic protein (ECP) and tryptase wereanalysed using commercially available fluoroimmunoassays (PharmaciaDiagnostics AB and Pharmacia & Upjohn, Uppsala, Sweden).ECP values <2 µg·L^–1 and tryptaselevels <1 µg·L^–1 were considerednegative. Eotaxin levels in BAL fluid were measured by enzyme-linkedimmunosorbent assay according to the manufacturer's description(Quantikine; R&D Systems, Minneapolis, MN, USA).

Statistical analysis
The data are presented as medians with lower and upper quartilevalues (P25–P75) unless otherwise stated. For intraindividualcomparisons of data retrieved before and after allergen challenge,Wilcoxon's signed-rank test was used. Correlations were calculatedusing the Spearman R test.

Results

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Abstract
Material and methods
Results
Discussion
Acknowledgements
References

Cornstarch glove powder exposure
The total dust concentration of cornstarch glove powder measuredon both sides close to the breathing zone of the subject was5.9 mg·m^–3 (interquartile range 5.5–6.2),and the concentration of respirable dust was 0.62 mg·m^–3(0.60–0.67). The airborne respirable dust was found tocontain $~$ 40% organic material, i.e. cornstarch, while the remainingfraction was MgO.

Bronchoalveolar lavage fluid cell counts
BAL fluid cells were retrieved and counted from all individualsbefore and after cornstarch glove powder exposure (table 1).The exposure resulted in a three-fold increase in BAL totalcell concentrations, from 84.2 to 241.3x10⁶ cells·L^–1(fig. 1a and table 1). There was a significant increasein concentrations of AM, lymphocytes and eosinophils, as wellas a strong tendency for mast cells, while neutrophils did notchange. Analysing relative numbers showed, however, that theonly cells with a significant increase were the eosinophils(fig. 1b), while macrophages were found to decrease significantly(table 1). Four individuals (subject nos 4, 6, 7 and 9)were evaluated at a third occasion, 7–8 months after thedust exposure. At that point, BAL fluid cells were close tothe original pre-exposure levels, with relative numbers of eosinophilsbeing 0.4, 0.4, 0 and 0.2%, respectively (fig. 1b).

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Table 1 Differential counts of bronchoalveolar lavage (BAL) fluid cells retrieved from 10 healthy individuals 2–3 weeks before and 1 day after exposure to cornstarch

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Fig. 1.— a) Bronchoalveolar lavage cell concentrations (x10⁶ L^–1) before and after cornstarch glove powder exposure in 10 healthy individuals and b) relative numbers (%) of eosinophil granulocytes 2–3 weeks before (n=10), 1 day after (n=10) and at follow-up 7–8 months after (n=4) exposure. Subject nos: ${diamondsuit}$ : 1; ${blacktriangledown}$ : 2; ${circ}$ : 3; ${triangleup}$ : 4; ${blacktriangleup}$ : 5; ${square}$ : 6; ${blacksquare}$ : 7; ${triangledown}$ : 8; •: 9; ${diamond}$ : 10. **: p<0.01.

ECP in BAL fluid was not detectable before dust exposure (<2 µg·mL^–1in all individuals), while after exposure four individuals (subjectnos 4, 6, 8 and 9) had elevated values (14, 0, 5.2, 2.2 and4.0, respectively). The postexposure ECP values in BAL fluidcorrelated significantly with the postexposure relative numbersof BAL eosinophils (p=0.01; fig. 2

). Tryptase was not detectedin BAL fluid, either before or after exposure. The eotaxin levelsin BAL fluid were similar before (42.7, 41.3–43.6 pg·mL^–1)and after exposure (41.3, 40.5–44.4 pg·mL^–1).

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Fig. 2.— Correlation between relative numbers of eosinophil granulocytes and eosinophil cationic protein (ECP) 1 day after exposure to cornstarch glove powder. BAL: bronchoalveolar lavage.

Alveolar macrophage phenotype
The AM expression of adhesion, activation and subset markerswas investigated in BAL fluid retrieved before and after dustexposure, and in addition in four individuals 7–8 monthsafter exposure (table 2

). The most distinct changes werenoted for the lipopolysaccharide receptor, CD14, which was expressedmore significantly by the AMs after exposure (p<0.01; fig.3a

), and for the Fc ${gamma}$ -receptor CD16, with a significantly reducedexpression after exposure (p=0.01; fig. 3b

). As can be notedin figure 3

, the expression of CD14 and CD16 tended toreturn to close to pre-exposure values when analysed again 7–8months after exposure. Both activation markers HLA class I andII were significantly reduced following exposure (table 2

).Markers for cell adhesion (CD11 and CD54) and costimulation(CD86) showed no significant changes (table 2

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Table 2 Expression of surface markers by alveolar macrophages from 10 individuals 2–3 weeks before and 1day [PDB] after exposure to corn dust

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Fig. 3.— Alveolar macrophages (AM) expression of a) CD14 or b) CD16 2–3 weeks before, 1 day after and at follow-up 7–8 months after exposure for cornstarch glove powder. AM expression is shown as mean fluorescence intensity (MFI). Subject nos: ${blacktriangledown}$ : 2; ${circ}$ : 3; ${triangleup}$ : 4; ${blacktriangleup}$ : 5; ${square}$ : 6; ${blacksquare}$ : 7; ${triangledown}$ : 8; •: 9; ${diamond}$ : 10. **: p<0.01.

Lymphocyte phenotype
Following starch exposure, the BAL CD4/CD8 ratio increased from1.4 to 3.4 (ns), indicating an influx of CD4+ T-cells into thealveoli. A careful phenotypic characterisation of CD4+ and CD8+lymphocyte subsets in BAL fluid as well as in peripheral bloodwas performed before and after dust exposure (table 3

).The most significant changes were found in the CD4+ BAL T-cellsubset, where the number of cells expressing an early activationmarker (CD69, p<0.01; fig. 4

), a late activation marker(HLA-DR, p<0.05) and a subset marker (CD57, p=0.01) significantlydecreased. Conversely, CD4+ BAL T-cells expressing the costimulatorymolecule CD28, increased significantly (p<0.05). Anotherearly activation marker, CD25, tended to be expressed by moreCD4+ BAL T-cells after exposure, while the number of cells expressingthe activation marker CD26 was unchanged (table 3

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Table 3 Phenotyping of CD4+ and CD8+ bronchoalveolar lavage (BAL) lymphocytes retrieved 2–3 weeks before and 1 day after exposure to cornstarch glove powder

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Fig. 4.— The relative numbers of CD4+ bronchoalveolar lavage (BAL) T-cells expressing CD69 2–3 weeks before, 1 day after and at follow-up 7–8 months after exposure for cornstarch glove powder. Subject nos: ${diamondsuit}$ : 1; ${blacktriangledown}$ : 2; ${circ}$ : 3; ${triangleup}$ : 4; ${blacktriangleup}$ : 5; ${square}$ : 6; ${blacksquare}$ : 7; ${triangledown}$ : 8; •: 9; ${diamond}$ : 10. **: p<0.01.

Similar to BAL CD4+ T-cells, the number of BAL CD8+ T-cellsexpressing CD69 was also significantly decreased after dustexposure (table 3

). In the BAL CD8+ T-cell subset, theonly other significant change was an increased number of T-cellsexpressing the activation marker CD26. The same marker was expressedby significantly more peripheral blood CD4+ T-cells (p<0.05)as well as CD8+ T-cells (p<0.05) after dust exposure, whileall other markers (CD25, CD28, CD57, CD69 and HLA-DR) were unchangedin both (CD4+ and CD8+) peripheral blood T-cell subsets.

To investigate any accumulation of antigen-specific T-cellsto the lungs, the relative numbers of T-cell receptor AV2S3,BV2 and BV8 expressing T-cells in the CD4+ and CD8+ BAL andperipheral blood T-cell subsets, respectively, were evaluatedin three individuals (subject nos 8, 9 and 10). In general,only minor changes were noted in each subset. The most pronouncedchange was found in individual 9, who had a CD4+ BAL T-cellexpansion expressing BV2 and making up 34.0% of all CD4+ BALT-cells. This T-cell expansion was reduced to 22.8% followingdust exposure, in line with an influx of polyclonal T-cellsexpressing other T-cell receptor variable (TCR V) gene segments.

Discussion

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Abstract
Material and methods
Results
Discussion
Acknowledgements
References

Since wheat flour is known to be an occupational allergen causingchronic respiratory disorders 1, the authors were interestedin understanding what roles different wheat flour componentsmay play in inducing airway inflammatory parameters. In thisstudy, the authors focused on starch, which is one ingredientin wheat flour. Cornstarch glove powder has been shown previouslyto be able to cause granulomatous inflammation 3, 4. To investigateany role for cornstarch in affecting airway inflammatory parameters,healthy individuals were exposed to cornstarch glove powder,using a whole-body exposure chamber, which was previously shownto provide a stable wheat aerosol concentration level insidethe chamber 2. Before and after exposure, BAL cell subpopulationswere analysed and in particular, using fluorescence-activatedcell sorter (FACS), the expression of various activation, adhesionand subset markers on AM and on BAL CD4+ and CD8+ T-cells wereinvestigated.

Dramatic changes in the BAL cell compartments were found afterexposure to cornstarch glove powder, with a three-fold increase(median) in the BAL cell concentration. The most intriguingfinding, however, was the select accumulation of eosinophilicgranulocytes, with increased relative numbers of eosinophilsin the BAL cell population in every individual. In fact, aftercornstarch glove powder exposure the eosinophils made up >10%of all BAL cells in four individuals, and $~$ 30% in two of theseindividuals. Furthermore, the significant correlation betweenrelative numbers of eosinophils and ECP suggests that the lung-accumulatedeosinophils were activated.

According to the manufacturer, the total cornstarch glove powderconsisted of cornstarch and a minor fraction of MgO, while therespirable dust was made up of $~$ 40% organic (cornstarch) and60% inorganic materials (MgO). The described inflammatory findingstherefore could possibly be induced by either of these components.Although Kuschner et al. 8 used a somewhat different form ofexposure compared with this study, using a freshly generatedMgO fume, they found no measurable pulmonary inflammatory response,with similar BAL cell concentrations and cytokine levels beforeand after MgO exposure. Also, the presence of MgO in cornstarchglove powder did not induce any detectable changes when analysingthe tissue response to surgical cornstarch glove powder in rats9. The authors consequently suggest that the organic fractionof glove powder is the active component to induce the eosinophilicgranulocyte accumulation in BAL fluid. In preliminary experimentsit was investigated whether cornstarch could affect eosinophiladhesion and/or transmigration, using a newly developed in vitromodel 10. However, in two separate experiments, any influenceof cornstarch on either interleukin-5-primed or unprimed eosinophilscould not be detected. An alternative mechanism may be thatcornstarch stimulated the release of chemoattractant factorsspecific for eosinophils, such as eotaxin 11, leading to a selectaccumulation of eosinophils in the BAL fluid. Eotaxin levelsin BAL fluid, however, were not found to change significantlyafter exposure.

Markers for monocyte/macrophage differentiation, adhesion andactivation were also analysed and it was found that the AM expressionof the lipopolysaccharide receptor CD14 was significantly increasedafter exposure, while CD16 (Fc ${gamma}$ RIII) and activation markers HLAclass I and class II molecules were significantly decreased.This finding is compatible with an influx to the airways ofmonocytes, with a higher expression of CD14 and a lower expressionof CD16 and HLA class I and II molecules compared with matureAMs 12–14. In healthy individuals, exposure to cornstarchglove powder thus results in an increased AM concentration inBAL fluid as well as an altered AM phenotype, consistent withan increased proportion of less activated and differentiatedmonocytic cells.

The BAL T-cell compartment also underwent significant changesafter cornstarch glove powder exposure. The most dramatic consequencewas the reduced number of CD4+ T-cells expressing the earlyactivation marker CD69, found in every individual. Moreover,the late activation marker HLA-DR was significantly reducedafter exposure, as was the relative number of C57+ T-cells,while CD28+ BAL CD4+ T-cells increased significantly. The authorshave previously described that CD69, HLA-DR and CD57 are expressedin relatively lower numbers and CD28 in relatively higher numbersin peripheral blood compared with BAL fluid CD4+ T-cells inhealthy individuals 15. The described changes after cornstarchglove powder exposure in the BAL CD4+ T-cell compartment aretherefore in congruence with an influx of peripheral blood T-cellsinto the alveoli. In addition, the finding of an essentiallysimilar expression of the three TCR V gene products analysedbefore and after exposure on BAL and peripheral blood T-cells,is also in line with an influx of a heterogeneous polyclonalT-cell population to the lungs.

Finally, the BAL cell differential counts and FACS analysiswere repeated 7–8 months after the cornstarch glove powderexposure in the four individuals with the most pronounced alterationsin the eosinophil distributions. At this time point there wasa complete normalisation with values close to identical to thoseobtained before exposure. Also, the FACS analyses suggesteda normalisation of the expression of markers on both AM andT-lymphocytes. Thus, the cornstarch glove powder exposure inducedonly a transiently altered BAL cell composition. Although clinicalparameters of bronchoconstriction or other airway symptoms werenot monitored, none of the individuals had any subjective complaintsof any symptoms at all. This result is in line with a previousreport showing no airway reaction after bronchial provocationswith nebulised cornstarch powder 6.

In conclusion, a whole-body exposure chamber was used to expose10 healthy individuals to cornstarch glove powder. Dramaticchanges in the bronchoalveolar lavage cell compartment werefound, with a three-fold increase in bronchoalveolar lavagecell concentrations. There was a selective accumulation andactivation of eosinophilic granulocytes, and an influx of peripheralblood derived monocytes and heterogeneous T-lymphocytes. Althougha normalisation was observed, the consequences of repeated exposurecannot be evaluated from this study with a single exposure.Cornstarch glove powder exposure may be an interesting modelfor future studies of lung-accumulated eosinophil granulocytesin humans.

Acknowledgements

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Abstract
Material and methods
Results
Discussion
Acknowledgements
References

The authors would like to thank B. Dahlberg, M. Dahl and G.de Forest for skillful technical assistance, and J. Lundahlfor discussions.

References

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Abstract
Material and methods
Results
Discussion
Acknowledgements
References

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