Type 2 Innate Lymphoid Cells in Severe Pediatric Asthma (CLASSE)
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| ClinicalTrials.gov Identifier: NCT03784781 |
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Recruitment Status : Unknown
Verified December 2018 by Assistance Publique - Hôpitaux de Paris.
Recruitment status was: Recruiting
First Posted : December 24, 2018
Last Update Posted : December 24, 2018
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| Condition or disease | Intervention/treatment |
|---|---|
| Severe Asthma | Biological: Biopsy Biological: Blood collection Biological: Bronchoalveolar lavage |
Severe asthma of the child is characterized by chronic eosinophilic infiltration of the bronchial mucosa associated with bronchial remodeling.
The mechanisms responsible for these phenomena are still misunderstood. Animal models suggest that type 2 innate lymphoid cells (ILC2) may be responsible for inflammation and bronchial remodeling in asthma. In mice, ILC2 stimulated by the pulmonary epithelium by viral aggression or allergenic exposure release cytokines of the TH2 type such as IL-5 and IL-13 and amphiregulin, involved in the recruitment and differentiation of eosinophils, bronchoconstriction, mucus secretion and the restoration of epithelial integrity.
In humans, ILC2 would be more abundant in the bronchoalveolar lavage (BAL) and peripheral blood of asthmatic patients compared to control subjects. However, the presence of ILC2 in the bronchial mucosa of asthmatic patients has never been identified.
The hypothesis tested is that ILC2 are more abundant in bronchial mucosa, BAL, and blood in children with severe asthma than in non-asthmatics. The results of this study would improve the knowledge of the mechanisms responsible for bronchial inflammation in asthma, consider therapies to prevent its development and modify the natural history of the disease.
The main objectives of this study are to show that the number of ILC2 in bronchial mucosa and BAL is higher in asthmatic children than in non-asthmatics, that the number of ILC2 in the bronchial mucosa and BAL is correlated with the number of eosinophils in bronchial mucosa and BAL, to determine whether the number of ILC2 in lungs correlate with asthma symptoms, and to determine whether there is a correlation between plasma and bronchial ILC2.
Bronchoscopy with BAL and bronchial mucosal biopsies will be performed in 20 children with severe asthma and 20 control subjects in the department of pediatric pulmonology and allergy of Necker Hospital.
ILC2 will be identified in the BAL, in the bronchial mucosa and peripheral blood by flow cytometry. The median values of the number of ILC2 will be compared between asthmatic and non-asthmatic patients by the Mann-Whitney non-parametric test. The correlations will be established by the Spearman rank test. A value of p < 0.05 will be considered significant.
| Study Type : | Observational |
| Estimated Enrollment : | 40 participants |
| Observational Model: | Case-Control |
| Time Perspective: | Cross-Sectional |
| Official Title: | Type 2 Innate Lymphoid Cells in Severe Pediatric Asthma |
| Actual Study Start Date : | June 9, 2016 |
| Estimated Primary Completion Date : | April 2020 |
| Estimated Study Completion Date : | April 2020 |
| Group/Cohort | Intervention/treatment |
|---|---|
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Asthmatic children
Severe uncontrolled asthma is defined by the need to maintain a treatment with high doses of inhaled corticosteroids and a long-acting bronchodilator (B2LDA) and/or an anti-leukotriene
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Biological: Biopsy
Mucosal biopsies under general anesthesia of the segmental bronchi of the right or left lower lobe Biological: Blood collection Blood collection (+15mL/ current care) Biological: Bronchoalveolar lavage Bronchoalveolar lavage fluid (3mL/Kg) |
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Controls
Non-asthmatic children, paired in age, requiring bronchial endoscopy with BAL and bronchial mucosa biopsy.
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Biological: Biopsy
Mucosal biopsies under general anesthesia of the segmental bronchi of the right or left lower lobe Biological: Blood collection Blood collection (+15mL/ current care) Biological: Bronchoalveolar lavage Bronchoalveolar lavage fluid (3mL/Kg) |
- Number of type 2 innate lymphoid cells [ Time Frame: Day 0 ]Type 2 innate lymphoid cells
- Number of Eosinophils [ Time Frame: Day 0 ]Eosinophils
- Airway remodeling: reticular basement membrane thickness [ Time Frame: Day 0 ]Reticular basement membrane thickness will be expressed in µm.
- Airway remodeling: airway smooth muscle area [ Time Frame: Day 0 ]The percentage of the submucosa occupied by airway smooth muscle will be determined on hematoxylin-eosin-stained and anti-airway smooth muscle antibody treated sections, respectively. The bundles of airway smooth muscle will be enclosed by a line and the area they occupied will be calculated by image analysis. The airway smooth muscle area will be expressed as the percentage of surface of the submucosa occupied by airway smooth muscle.
- Airway remodeling: epithelial integrity [ Time Frame: Day 0 ]Epithelial integrity will be defined as the percentage of the total length of epithelium that will be intact.
- Airway remodeling: vessel number [ Time Frame: Day 0 ]The number of vessels stained with anti-CD31 mAb will be determined from at least one grid (0.1 mm2) per biopsy, and reported as the median number of positive sections per 0.1 mm2.
- Airway remodeling: mucus gland area [ Time Frame: Day 0 ]The percentage of the submucosa occupied by mucus gland will be determined on hematoxylin-eosin-stained and anti-airway smooth muscle antibody treated sections, respectively. The mucus glands will be enclosed by a line and the area occupied will be calculated by image analysis. The mucus gland area will be expressed as the percentage of surface of the submucosa occupied by mucus gland.
- Airway inflammation: bronchoalveolar lavage (BAL) [ Time Frame: Day 0 ]
BAL fluid will be assed for inflammation
- The number of eosinophils will be assessed and expressed percentage of total cells in BAL
- The number of neutrophils will be assessed and expressed percentage of total cells in BAL
- The number of macrophages will be assessed and expressed percentage of total cells in BAL
- The number of basophils will be assessed and expressed percentage of total cells in BAL
- The number of mast cells will be assessed and expressed percentage of total cells in BAL
- The number of innate lymphoid cells will be assessed and expressed percentage of total cells in BAL
- The number of mucosal associated invariant T (MAIT) cells will be assessed and expressed percentage of total cells in BAL
- The number of invariant natural killer T cells will be assessed and expressed percentage of total cells in BAL
- The number of gammadelta T cells will be assessed and expressed percentage of total cells in BAL
- Airway inflammation: bronchial mucosa [ Time Frame: Day 0 ]
Bronchial sections will be stained with May-Grunwald-Giemsa.The number of inflammatory cells will be assessed in the submucosa and expressed as the number of cells per square millimeters of submucosal area.
- The number of eosinophils will be assessed and expressed per square millimeters of submucosal area
- The number of neutrophils in the submucosa will be assessed and expressed per square millimeters of submucosal area
- The number of mast cells (c-kit positive cells) in the submucosa will be assessed and expressed per square millimeters of submucosal area
- The number of IgE stained with anti-IgE Ab in the submucosa and the epithelium will be assessed and expressed per square millimeters of submucosal area
- The expression of cytokines in the mucosa will be assessed by multiplex
- Inflammation in blood [ Time Frame: Day 0 ]
- The number of eosinophils will be assessed and expressed percentage of total cells in blood
- The number of neutrophils will be assessed and expressed percentage of total cells in blood
- The number of basophils will be assessed and expressed percentage of total cells in blood
- The number of lymphocytes will be assessed and expressed percentage of total cells in blood
- The number of innate lymphoid cells will be assessed and expressed percentage of total cells in blood
- The number of mucosal associated invariant T (MAIT) cells will be assessed and expressed percentage of total cells and T cells in blood
- The number of invariant natural killer T cells will be assessed and expressed percentage of total cells and T cells in blood
- The number of gammadelta T cells will be assessed and expressed percentage of total cells and T cells in blood
- The expression of cytokine will be assessed using multiplex analysis
- Metabolomic signature [ Time Frame: Day 0 ]Non-targeted metabolomics analysis will be performed on plasma. Metabolic profiles will be obtained using two complementary LC-MS methods, to identify metabolites discriminating different patients.
- Microbiota analysis [ Time Frame: Day 0 ]Microbiota analysis will be performed on BAL using PCR ARN 16S.
Biospecimen Retention: Samples With DNA
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| Ages Eligible for Study: | 6 Years to 18 Years (Child, Adult) |
| Sexes Eligible for Study: | All |
| Accepts Healthy Volunteers: | No |
| Sampling Method: | Non-Probability Sample |
Inclusion Criteria:
Controls :
- Minors aged 6 to 18 matched in age with severe asthmatic children
- Non-asthmatic children hospitalized in the department of pediatric pulmonology and allergy in Necker Hospital
- To undergo bronchial endoscopy with bronchoalveolar lavage, biopsy and blood collection
Severe asthmatic children :
- Minors aged 6 to 18
- Children hospitalized in the department of pediatric pulmonology and allergy in Necker Hospital
- To undergo bronchial endoscopy with bronchoalveolar lavage, biopsy and blood collection
- Severe uncontrolled asthma is defined by the need to maintain a treatment with high doses of inhaled corticosteroids and a long-acting bronchodilator (B2LDA) and/or an anti-leukotriene
Exclusion Criteria:
- Children with an immune deficiency, will be excluded
To learn more about this study, you or your doctor may contact the study research staff using the contact information provided by the sponsor.
Please refer to this study by its ClinicalTrials.gov identifier (NCT number): NCT03784781
| Contact: Guillaume Lezmi, MD, PhD | +33 1 44 49 48 38 | guillaume.lezmi@aphp.fr | |
| Contact: Hélène Morel | +33 1 44 38 16 53 | helene.morel@aphp.fr |
| France | |
| Hôpital Necker Enfants malades | Recruiting |
| Paris, France, 75015 | |
| Contact: Guillaume Lezmi, MD, PhD +33 1 44 49 48 38 guillaume.lezmi@aphp.fr | |
| Principal Investigator: | Guillaume Lezmi, MD, PhD | Assistance Publique - Hôpitaux de Paris |
| Responsible Party: | Assistance Publique - Hôpitaux de Paris |
| ClinicalTrials.gov Identifier: | NCT03784781 |
| Other Study ID Numbers: |
APHP180357 |
| First Posted: | December 24, 2018 Key Record Dates |
| Last Update Posted: | December 24, 2018 |
| Last Verified: | December 2018 |
| Individual Participant Data (IPD) Sharing Statement: | |
| Plan to Share IPD: | No |
| Studies a U.S. FDA-regulated Drug Product: | No |
| Studies a U.S. FDA-regulated Device Product: | No |
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Severe asthma in children Type 2 innate lymphoid cells (ILC2) bronchial mucosa bronchoalveolar lavages |
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Asthma Bronchial Diseases Respiratory Tract Diseases Lung Diseases, Obstructive Lung Diseases |
Respiratory Hypersensitivity Hypersensitivity, Immediate Hypersensitivity Immune System Diseases |