Weight loss and lipolysis promote a dynamic immune response in murine adipose tissue
Aliki Kosteli, … , Rudolf Zechner, Anthony W. Ferrante Jr.
Aliki Kosteli, … , Rudolf Zechner, Anthony W. Ferrante Jr.
Published September 27, 2010
Citation Information: J Clin Invest. 2010;120(10):3466-3479. https://doi.org/10.1172/JCI42845.
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Research Article

Weight loss and lipolysis promote a dynamic immune response in murine adipose tissue

Abstract

Obesity elicits an immune response characterized by myeloid cell recruitment to key metabolic organs, including adipose tissue. However, the response of immune cells to nonpathologic metabolic stimuli has been less well studied, and the factors that regulate the metabolic-dependent accumulation of immune cells are incompletely understood. Here we characterized the response of adipose tissue macrophages (ATMs) to weight loss and fasting in mice and identified a role for lipolysis in ATM recruitment and accumulation. We found that the immune response to weight loss was dynamic; caloric restriction of high-fat diet–fed mice led to an initial increase in ATM recruitment, whereas ATM content decreased following an extended period of weight loss. The peak in ATM number coincided with the peak in the circulating concentrations of FFA and adipose tissue lipolysis, suggesting that lipolysis drives ATM accumulation. Indeed, fasting or pharmacologically induced lipolysis rapidly increased ATM accumulation, adipose tissue chemoattractant activity, and lipid uptake by ATMs. Conversely, dietary and genetic manipulations that reduced lipolysis decreased ATM accumulation. Depletion of macrophages in adipose tissue cultures increased expression of adipose triglyceride lipase and genes regulated by FFA, and increased lipolysis. These data suggest that local lipid fluxes are central regulators of ATM recruitment and that once recruited, ATMs form lipid-laden macrophages that can buffer local increases in lipid concentration.

Authors

Aliki Kosteli, Eiji Sugaru, Guenter Haemmerle, Jayne F. Martin, Jason Lei, Rudolf Zechner, Anthony W. Ferrante Jr.

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Figure 9

Adipose tissue explants were isolated from high-fat diet–induced obese mice that were fasting for 24 hours.

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Adipose tissue explants were isolated from high-fat diet–induced obese m...
Subsequently, explants were treated either with liposome-encapsulated clodronate or liposome-encapsulated PBS. Explants from the same mice were treated with both experimental conditions. (A) Gene expression of macrophage-specific genes and genes involved in lipid metabolism in the explants. Data are represented as mean ± SD. n = 4 mice/group. (B) Glycerol release from explants of perigonadal adipose tissue treated either with liposome-encapsulated clodronate or liposome-encapsulated PBS. Liposome-encapsulated clodronate was administered intraperitoneally to lean C57BL/6J mice. Mice were fasted for 24 hours starting on day 3 after injection, and macrophage depletion in perigonadal adipose tissue was confirmed at the end of the fasting period (day 4). Liposome-encapsulated PBS was also administered as control. (C) Serum concentration of FFA in clodronate- or PBS-treated mice after a 24-hour fast. Data are represented as mean ± SD. n = 8 mice/group. *P < 0.05; **P < 0.01, versus PBS treated.