Protocol for phenotyping and isolation of dendritic cell subsets from blood and lymphoid organs of non-human primates and humans by flow cytometry
Juliette Pons, Margaux Gardet, Florian Meurisse, Francis Relouzat, Olivier Lambotte, Benoit Favier

TL;DR
This paper provides a detailed protocol for isolating and analyzing dendritic cell subsets from blood and lymphoid organs of non-human primates and humans using flow cytometry.
Contribution
The paper introduces a comprehensive and optimized protocol for ex vivo phenotyping and purification of dendritic cell subsets using flow cytometry.
Findings
Steps for isolating mononuclear cells from blood, lymph nodes, and spleen are detailed.
Optimized antibody panels are provided for identifying DC subsets via flow cytometry.
Protocols for cytokine production analysis and high-purity sorting of DC subsets are described.
Abstract
Dendritic cells (DCs) encompass several subsets that are essential for shaping immune responses. Here, we present a protocol for ex vivo functional analysis and purification of DC subsets from blood and secondary lymphoid organs using flow cytometry. We describe the steps for isolating mononuclear cells from blood, lymph nodes, and spleen. We then detail the procedures for phenotypic characterization of DC subsets, intracellular staining to assess their cytokine production, and fluorescence-activated cell sorting (FACS) to isolate individual DC populations. For complete details on the use and execution of this protocol, please refer to Gardet et al.1 •Steps for isolating a single-cell suspension from blood, lymph nodes, and spleen of NHP•Guidance on identifying DC subsets via flow cytometry with optimized antibody panels•Steps for ex vivo stimulation and analysis of cytokine…
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Taxonomy
TopicsImmunotherapy and Immune Responses · T-cell and B-cell Immunology · Immune Cell Function and Interaction
