Standardized high‐dimensional spectral cytometry protocol and panels for whole blood immune phenotyping in clinical and translational studies

Author:

Dott Tom12,Culina Slobodan1,Chemali Rene1,Mansour Cedric Ait3,Dubois Florian12,Jagla Bernd14,Doisne Jean Marc5,Rogge Lars6,Huetz François7,Jönsson Friederike78,Commere Pierre‐Henri1,Di Santo James5,Terrier Benjamin9,Quintana‐Murci Lluis10,Duffy Darragh12,Hasan Milena1ORCID,

Affiliation:

1. Cytometry and Biomarkers UTechS, Institut Pasteur Université Paris Cité Paris France

2. Translational Immunology Unit Institut Pasteur, Université Paris Cité Paris France

3. Sony Europe BV Surrey UK

4. Bioinformatics and Biostatistics Hub, Institut Pasteur Université Paris Cité Paris France

5. Innate Immunity Unit, Institut Pasteur Université Paris Cité Paris France

6. Immunoregulation Unit, Institut Pasteur Université Paris Cité Paris France

7. Unit of Antibodies in Therapy and Pathology, INSERM UMR1222, Institut Pasteur Université de Paris Cité Paris France

8. CNRS Paris France

9. Service de Médecine Interne Hôpital Cochin Paris France

10. Human Evolutionary Genetics Unit, CNRS, Institut Pasteur Université Paris Cité, UMR2000 Paris France

Abstract

AbstractFlow cytometry is the method of choice for immunophenotyping in the context of clinical, translational, and systems immunology studies. Among the latter, the Milieu Intérieur (MI) project aims at defining the boundaries of a healthy immune response to identify determinants of immune response variation. MI used immunophenotyping of a 1000 healthy donor cohort by flow cytometry as a principal outcome for immune variance at steady state. New generation spectral cytometers now enable high‐dimensional immune cell characterization from small sample volumes. Therefore, for the MI 10‐year follow up study, we have developed two high‐dimensional spectral flow cytometry panels for deep characterization of innate and adaptive whole blood immune cells (35 and 34 fluorescent markers, respectively). We have standardized the protocol for sample handling, staining, acquisition, and data analysis. This approach enables the reproducible quantification of over 182 immune cell phenotypes at a single site. We have applied the protocol to discern minor differences between healthy and patient samples and validated its value for application in immunomonitoring studies. Our protocol is currently used for characterization of the impact of age and environmental factors on peripheral blood immune phenotypes of >400 donors from the initial MI cohort.

Funder

Agence Nationale de la Recherche

Publisher

Wiley

Subject

Cell Biology,Histology,Pathology and Forensic Medicine

Reference24 articles.

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4. Anon.10kimmunomes—Default. [cited 2023 May 30].https://comphealth.ucsf.edu/app/10kimmunomes

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