Differential importance of endothelial and hematopoietic cell GLP-1Rs for cardiometabolic versus hepatic actions of semaglutide
Brent A. McLean, … , Randy J. Seeley, Daniel J. Drucker
Brent A. McLean, … , Randy J. Seeley, Daniel J. Drucker
Published October 21, 2021
Citation Information: JCI Insight. 2021;6(22):e153732. https://doi.org/10.1172/jci.insight.153732.
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Research Article Endocrinology

Differential importance of endothelial and hematopoietic cell GLP-1Rs for cardiometabolic versus hepatic actions of semaglutide

Abstract

Glucagon-like peptide-1 receptor agonists (GLP-1RAs) are used to treat diabetes and obesity and reduce rates of major cardiovascular events, such as stroke and myocardial infarction. Nevertheless, the identity of GLP-1R–expressing cell types mediating the cardiovascular benefits of GLP-1RA remains incompletely characterized. Herein, we investigated the importance of murine Glp1r expression within endothelial and hematopoietic cells. Mice with targeted inactivation of Glp1r in Tie2+ cells exhibited reduced levels of Glp1r mRNA transcripts in aorta, liver, spleen, blood, and gut. Glp1r expression in bone marrow cells was very low and not further reduced in Glp1rTie2–/– mice. The GLP-1RA semaglutide reduced the development of atherosclerosis induced by viral PCSK9 expression in both Glp1rTie2+/+ and Glp1rTie2–/– mice. Hepatic Glp1r mRNA transcripts were reduced in Glp1rTie2–/– mice, and liver Glp1r expression was localized to γδ T cells. Moreover, semaglutide reduced hepatic Tnf, Abcg1, Tgfb1, Cd3g, Ccl2, and Il2 expression; triglyceride content; and collagen accumulation in high-fat, high-cholesterol diet–fed Glp1rTie2+/+ mice but not Glp1rTie2–/– mice. Collectively, these findings demonstrate that Tie2+ endothelial or hematopoietic cell GLP-1Rs are dispensable for the antiatherogenic actions of GLP-1RA, whereas Tie2-targeted GLP-1R+ cells are required for a subset of the antiinflammatory actions of semaglutide in the liver.

Authors

Brent A. McLean, Chi Kin Wong, Kiran Deep Kaur, Randy J. Seeley, Daniel J. Drucker

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Figure 5

Glp1r expression in the liver is localized to CD8α and γδ T cells.

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Glp1r expression in the liver is localized to CD8α and γδ T cells. (A) C...
(A) Cytometry gating strategy shown for liver T cell populations. (B) Whole liver (Liv), Percoll-purified nonhepatocyte cells (NH), and FACS-collected NH cells positive for CD3+TCRγδ or CD3+TCRβ (γδ-T) and either CD8α (CD8+) or CD4 (CD4+) were analyzed for expression of Glp1r as well as (C) Adgre1, Cd3g, Glp2r, and Crp as markers of macrophages, T cells, stellate cells, and hepatocytes, respectively, versus Tbp (n = 4–5). Data are presented as mean ± SD, with individual data points shown. (D) Full-length Glp1r transcript was amplified in liver as well as CD8+ and TCR γδ+ T cell populations; lung (Lng) and Brunner’s glands (BG) are positive controls (representative of 3 replicates). (E) IFN-γ (Ifng) expression in freshly isolated NH cells from Glp1rTie2+/+ (n = 7) and Glp1rTie2–/– (n = 6) mice were cultured overnight with CD3/CD28 stimulation with or without exendin-4 (Ex-4; 50 nM), negative isotype control (ISO), and PMA-ionomycin (PMA-I) positive control (n = 9). *P < 0.05 paired t test.