A Single-cell Approach to Identify Biomarkers of Efficacy and Toxicity for ICI in NSCLC
NCT ID: NCT04807114
Last Updated: 2024-07-01
Study Results
The study team has not published outcome measurements, participant flow, or safety data for this trial yet. Check back later for updates.
Basic Information
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RECRUITING
70 participants
OBSERVATIONAL
2020-02-01
2025-01-31
Brief Summary
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A second aim is to characterize the immune cell composition of bronchoalveolar lavage (BAL) fluid from these ICI-treated cancer patients if they would develop ICI-pneumonitis. These mechanistic insights can directly lead to putative diagnostic biomarkers and therpeutic targets. Since single-cell profiling of blood samples will also be performed, circulating biomarkers of ICI toxicity can also be identified, making non-invasive diagnosis feasible.
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Detailed Description
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First, scRNA-seq and TCR-seq will be applied on up to 5,000 randomly dissociated cells. Additionally, cell surface protein expression can be integrated with the transcriptional information. Various bioinformatics pipelines, including Seurat, will be used to identify different cell clusters, which through marker gene expression will be assigned to known cell types, cellular subtypes or phenotypes. For instance, this will enable the researchers to monitor the abundance of PD-1/PD-L1 expressing T cells, cytotoxic T-cells, immune-suppressive myeloid cells, etc. The following parameters at single-cell level will be relevant (non-exhaustive):
* The composition and relative abundancies of established immune cell types (e.g. T cells (CD4+, CD8+ and regulatory subsets), NK cells, B cells, MDSCs, macrophages, neutrophils, dendritic cells). Transcriptomic data for each of these immune cell subtypes will be analyzed, allowing characterization of specific gene expression programs that define specific phenotypic states.
* Composition of all stromal cellular subtypes identified by single-cell transcriptomics, including fibroblasts and endothelial cells.
* A gene regulatory network for each cell type and cellular subtype (or cell state) will be established and master transcriptional regulators will be identified. Individual T cells and T cell sub-clusters will be classified based on interferon activation, high rates of proliferation and transcription and increased granzyme expression, which are all indicative of T cell activation. Since high CD8+ T cell activity correlates with high immune checkpoint expression, T cell activity (based on granzyme expression) will be correlated with expression of other genes in these cells to identify co-regulated receptors, which possibly represent novel checkpoint molecules.
Blood samples will be subjected to similar experimental procedures. First, PBMC are isolated using Ficoll density gradient centrifugation. Single-cell transcriptome analysis in combination with CITE- seq will be performed on 5000 PBMC. Cellular composition will be determined using the same bioinformatic pipelines as used for processing the tumor biopsies.
As a second objective, immune profiling of the cellular composition of ICI-pneumonitis BAL fluid and PBMC will be performed using scRNA-seq, scTCR-seq and CITE-seq as previously outlined.
Conditions
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Study Design
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COHORT
PROSPECTIVE
Study Groups
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NSCLC st.IV (PD-L1 > 50%)
Anti-PD-1 monotherapy
Immune checkpoint inhibitor
Standard-of-care treatment for st.IV NSCLC (no driver mutation, PD-L1 \> 50%)
NSCLC st.IV (PD-L1 < 50%)
Combination anti-PD-1 + chemotherapy
Chemotherapy + Immune checkpoint inhibitor
Standard-of-care treatment for st.IV NSCLC (no driver mutation, PD-L1 \< 50%)
Interventions
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Immune checkpoint inhibitor
Standard-of-care treatment for st.IV NSCLC (no driver mutation, PD-L1 \> 50%)
Chemotherapy + Immune checkpoint inhibitor
Standard-of-care treatment for st.IV NSCLC (no driver mutation, PD-L1 \< 50%)
Other Intervention Names
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Eligibility Criteria
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Inclusion Criteria
* Histologically and clinically confirmed diagnosis of non-small cell lung cancer (according to IASLC Staging Handbook in Thoracic Oncology v7)
* Patients receiving first-line treatment per guidelines
* Not included in other clinical trials
* Signed informed consent form
Exclusion Criteria
18 Years
120 Years
ALL
No
Sponsors
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KU Leuven
OTHER
Universitaire Ziekenhuizen KU Leuven
OTHER
Responsible Party
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Principal Investigators
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Els Wauters, MD, PhD
Role: PRINCIPAL_INVESTIGATOR
University Hospitals - KU Leuven
Locations
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Universitaire Ziekenhuizen Leuven
Leuven, , Belgium
Countries
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Central Contacts
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Facility Contacts
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Other Identifiers
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S63531
Identifier Type: -
Identifier Source: org_study_id
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