Obesity results in adipose tissue T cell exhaustion
Cara E. Porsche, Jennifer B. Delproposto, Lynn Geletka, Robert O’Rourke, Carey N. Lumeng
Cara E. Porsche, Jennifer B. Delproposto, Lynn Geletka, Robert O’Rourke, Carey N. Lumeng
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Research Article Inflammation Metabolism

Obesity results in adipose tissue T cell exhaustion

Abstract

Despite studies implicating adipose tissue T cells (ATT) in the initiation and persistence of adipose tissue inflammation, fundamental gaps in knowledge regarding ATT function impedes progress toward understanding how obesity influences adaptive immunity. We hypothesized that ATT activation and function would have tissue-resident–specific properties and that obesity would potentiate their inflammatory properties. We assessed ATT activation and inflammatory potential within mouse and human stromal vascular fraction (SVF). Surprisingly, murine and human ATTs from obese visceral white adipose tissue exhibited impaired inflammatory characteristics upon stimulation. Both environmental and cell-intrinsic factors are implicated in ATT dysfunction. Soluble factors from obese SVF inhibit ATT activation. Additionally, chronic signaling from macrophage major histocompatibility complex II (MHCII) is necessary for ATT impairment in obese adipose tissue but is independent of increased PD1 expression. To assess intracellular signaling mechanisms responsible for ATT inflammation impairments, single-cell RNA sequencing of ATTs was performed. ATTs in obese adipose tissue exhibit enrichment of genes characteristic of T cell exhaustion and increased expression of coinhibitory receptor Btla. In sum, this work suggests that obesity-induced ATTs have functional characteristics and gene expression resembling T cell exhaustion induced by local soluble factors and cell-to-cell interactions in adipose tissue.

Authors

Cara E. Porsche, Jennifer B. Delproposto, Lynn Geletka, Robert O’Rourke, Carey N. Lumeng

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Figure 1

ATT activation capacity is dependent upon diet type.

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ATT activation capacity is dependent upon diet type. (A) Flow cytometry ...
(A) Flow cytometry gating strategy used for ATT activation assays. Plot shows eWAT SVF after 3 days of coculture with αCD3/CD28 Dynabeads. Gating is representative of all ATT activation assays. (B) Frequency of CD25 expression on Tconv, CD8+, and Tregs after T cell activation assays. T cells from splenocytes, oWAT SVF, and eWAT SVF cultures taken from ND- and HFD-fed mice after 18 weeks of feeding. (C) Frequency of Ki67 expression on Tconv, CD8+, and Tregs from splenocytes and eWAT after T cell activation assays. Cell fractions were assessed with or without αCD3/CD28 Dynabead coculture for 3 days. n = 4 biological replicates/group, analyzed by 2-way ANOVA where *P < 0.05, **P < 0.01, ****P < 0.0001. (D and E) Heatmap of luminex assessment of supernatants taken from T cell activation cultures after 3 days (D) and bar graph representation of IL-2, IFN-γ, IL-17, and IL-4 data (E) shown in D. n = 3 biological replicates/group, analyzed by 2-way ANOVA where *P < 0.05, **P < 0.01, ***P < 0.001.