Healthy Clinical Trial
— ILLUMINA-2Official title:
Pulmonary Immune Cell-microbiome Interactions in the Healthy Lung: The ILLUMINA-2 Study
The overall aim is to to provide a normal material for the composition and spatial heterogeneity of the following in the healthy lung: i) immune cell populations and their activation patterns, ii) the surrounding cytokine-chemokine milieu, including trans-compartmental fluxes of these mediators between the lung and bloodstream, and iii) the lung microbiome. Main hypotheses: - Absolute and relative immune cell counts in bronchoalveolar lavage fluid (BALF) are similar to those previously reported by other methods6,7. - No trans-compartmental flux of cytokines between the lungs and bloodstream is present, but cytokine concentrations (notably IL-6 and IL-8) vary with the immune-cell-microbiome composition. - Immune cell (mainly T cell) activation, differentiation, and gene expression patterns are expected to differ between blood and BALF in a manner that depends on the regional diversity of the pulmonary microbiome.
Status | Recruiting |
Enrollment | 50 |
Est. completion date | November 30, 2028 |
Est. primary completion date | November 30, 2028 |
Accepts healthy volunteers | |
Gender | All |
Age group | 40 Years to 75 Years |
Eligibility | Inclusion Criteria: - Men and women - Age 40 to 75 Exclusion Criteria: - Immune deficiency - Lung disease - Active cancer or infection - Absolute contraindications for bronchoscopy - Untreated malignant arrhythmia - Documented or suspected intracranial hypertension (intracranial pressure = > 15 mmHg) - One-lung ventilation - Severe coagulopathy |
Country | Name | City | State |
---|---|---|---|
Denmark | Hvidovre Hospital, University of Copenhagen | Hvidovre |
Lead Sponsor | Collaborator |
---|---|
Hvidovre University Hospital |
Denmark,
Type | Measure | Description | Time frame | Safety issue |
---|---|---|---|---|
Primary | Lung microbiome | 16S ribosomal RNA (rRNA) and 18S rRNA PCR for bacterial or fungal pathogen identification in bronchoalveolar lavage fluid | Day 0 (subsequent to study inclusion) | |
Primary | Lymphocyte populations | Cell populations and subpopulations evaluated by 10 colored flow cytometry (B cells, T cells, TCR subsets, Tregs/Th17, dendritic cells, myeloid cells and neutrophils) in bronchoalveolar lavage fluid and blood | Day 0 (subsequent to study inclusion) | |
Secondary | Cell differential counts and cytomorphological analyses of BALF | Day 0 (subsequent to study inclusion) | ||
Secondary | Trans-compartmental fluxes | (calculated from plasma- and urea-adjusted BAL) | Day 0 (subsequent to study inclusion) | |
Secondary | Auto-antibodies against tI-IFNs in blood | Measured in bronchoalveolar lavage fluid | Day 0 (subsequent to study inclusion) | |
Secondary | White blood cells counts | Total white blood cells, neutrocytes, lymphocytes, and monocytes in bronchoalveolar lavage fluid and blood | Day 0 (subsequent to study inclusion) | |
Secondary | Cytokines | Multiplex assay for measuring cytokines in bronchoalveolar lavage fluid and plasma (e.g. IL-1-beta, IL-1RA, IL-2, IL-6, IL-8, IL-10, IL-17, IL-18, IL-33, IL-35, TGF-beta, TNF-alpha, HMGB1) | Day 0 (subsequent to study inclusion) | |
Secondary | Number and characterizations of respiratory pathogens | Respiratory film array PCR for testing for number of pathogens | Day 0 (subsequent to study inclusion) | |
Secondary | Number and characterizations of microorganisms | Growth of pathogenic microorganisms in body fluids (e.g. urine, blood, bronchoalveolar lavage fluid) in microbiological assays | Up to 12 weeks |
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