Determination of Interleukin-17A and Interferon-γ Production in γδ, CD4+, and CD8+ T Cells Isolated from Murine Lymphoid Organs, Perivascular Adipose Tissue, Kidney, and Lung

被引:7
作者
Comeau, Kevin [1 ]
Caillon, Antoine [1 ]
Paradis, Pierre [1 ]
Schiffrin, Ernesto L. [1 ,2 ]
机构
[1] McGill Univ, Lady Davis Inst Med Res, Sir Mortimer B Davis Jewish Gen Hosp, Vasc & Hypertens Res Unit, Montreal, PQ, Canada
[2] McGill Univ, Sir Mortimer B Davis Jewish Gen Hosp, Dept Med, Montreal, PQ, Canada
基金
加拿大健康研究院;
关键词
T-cell activation; Intracellular staining; Flow cytometry; Cytokines; Phenotyping; Hypertension; II-INDUCED HYPERTENSION;
D O I
10.21769/BioProtoc.4679
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
T cells localized to the kidneys and vasculature/perivascular adipose tissue (PVAT) play an important role in hypertension and vascular injury. CD4(+), CD8(+), and.d T-cell subtypes are programmed to produce interleukin (IL)-17 or interferon-gamma (IFN gamma), and naive T cells can be induced to produce IL-17 via the IL-23 receptor. Importantly, both IL-17 and IFN gamma have been demonstrated to contribute to hypertension. Therefore, profiling cytokine-producing T-cell subtypes in tissues relevant to hypertension provides useful information regarding immune activation. Here, we describe a protocol to obtain single-cell suspensions from the spleen, mesenteric lymph nodes, mesenteric vessels and PVAT, lungs, and kidneys, and profile IL-17A- and IFN gamma-producing T cells using flow cytometry. This protocol is different from cytokine assays such as ELISA or ELISpot in that no prior cell sorting is required, and various T-cell subsets can be identified and individually assessed for cytokine production simultaneously within an individual sample. This is advantageous as sample processing is kept to a minimum, yet many tissues and T-cell subsets can be screened for cytokine production in a single experiment. In brief, single-cell suspensions are activated in vitro with phorbol 12-myristate 13-acetate (PMA) and ionomycin, and Golgi cytokine export is inhibited with monensin. Cells are then stained for viability and extracellular marker expression. They are then fixed and permeabilized with paraformaldehyde and saponin. Finally, antibodies against IL-17 and IFN gamma are incubated with the cell suspensions to report cytokine production. T-cell cytokine production and marker expression is then determined by running samples on a flow cytometer. While other groups have published methods to perform T-cell intracellular cytokine staining for flow cytometry, this protocol is the first to describe a highly reproducible method to activate, phenotype, and determine cytokine production by CD4, CD8, and gamma delta T cells isolated from PVAT. Additionally, this protocol can be easily modified to investigate other intracellular and extracellular markers of interest, allowing for efficient T-cell phenotyping.
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页数:21
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