Polarization of M1 and M2 Human Monocyte-Derived Cells and Analysis with Flow Cytometry upon Mycobacterium tuberculosis Infection

Akhirunnesa Mily; Sadaf Kalsum; Marco Giulio Loreti; Rokeya Sultana Rekha; Jagadeeswara Rao Muvva; Magda Lourda; Susanna Brighenti

doi:10.3791/61807

Polarization of M1 and M2 Human Monocyte-Derived Cells and Analysis with Flow Cytometry upon Mycobacterium tuberculosis Infection

J Vis Exp. 2020 Sep 18:(163). doi: 10.3791/61807.

Authors

Akhirunnesa Mily¹, Sadaf Kalsum², Marco Giulio Loreti², Rokeya Sultana Rekha³, Jagadeeswara Rao Muvva², Magda Lourda⁴, Susanna Brighenti²

Affiliations

¹ Center for Infectious Medicine (CIM), Department of Medicine Huddinge, ANA Futura, Karolinska Institutet; Infectious Diseases Division, International Centre for Diarrhoeal Disease Research, Bangladesh ;mily.akhirunnesa@ki.se.
² Center for Infectious Medicine (CIM), Department of Medicine Huddinge, ANA Futura, Karolinska Institutet.
³ Clinical Microbiology, Department of Laboratory Medicine (Labmed), ANA Futura, Karolinska Institutet.
⁴ Center for Infectious Medicine (CIM), Department of Medicine Huddinge, ANA Futura, Karolinska Institutet; Childhood Cancer Research Unit, Department of Women's and Children's Health, Karolinska Institutet.

PMID: 33016941
DOI: 10.3791/61807

Abstract

Human macrophages are primary host cells of intracellular Mycobacterium tuberculosis (Mtb) infection and thus have a central role in immune control of tuberculosis (TB). We have established an experimental protocol to follow immune polarization of myeloid-derived cells into M1 (classically activated) or M2 (alternatively activated) macrophage-like cells through assessment with a 10-color flow cytometry panel that allows visualization and deep-characterization of green-fluorescent-protein (GFP)-labeled Mtb in diverse macrophages subsets. Monocytes obtained from healthy blood donors were polarized into M1 or M2 cells using differentiation with granulocyte macrophage-colony-stimulating factor (GM-CSF) or macrophage-colony stimulating factor (M-CSF) followed by polarization with IFN-γ and lipopolysaccharide (LPS) or IL-4, respectively. Fully polarized M1 and M2 cells were infected with Mtb-GFP for 4 hours before detached Mtb-infected macrophages were stained with flow cytometry at 4- or 24-hours post-infection. Sample acquisition was performed with flow cytometry and the data was analyzed using a flow cytometry analysis software. Manual gating as well as dimensionality reduction with Uniform Manifold Approximation and Projection (UMAP) and phenograph analysis was performed. This protocol resulted in effective M1/M2 polarization characterized by elevated levels of CD64, CD86, TLR2, HLA-DR and CCR7 on uninfected M1 cells, while uninfected M2 cells exhibited a strong up-regulation of the M2 phenotype markers CD163, CD200R, CD206 and CD80. M1-polarized cells typically contained fewer bacteria compared to M2-polarized cells. Several M1/M2 markers were downregulated after Mtb infection, which suggests that Mtb can modulate macrophage polarization. In addition, 24 different cell clusters of different sizes were found to be uniquely distributed among the M1 and M2 uninfected and Mtb-infected cells at 24-hours post-infection. This M1/M2 flow cytometry protocol could be used as a backbone in Mtb-macrophage research and be adopted for special needs in different areas of research.

Publication types

Research Support, Non-U.S. Gov't
Video-Audio Media

MeSH terms

Biomarkers / metabolism
Cell Polarity*
Cells, Cultured
Flow Cytometry / methods*
Humans
Macrophages / cytology*
Macrophages / immunology
Macrophages / metabolism
Monocytes / cytology*
Tuberculosis / immunology*
Tuberculosis / metabolism

Substances

Biomarkers