Adipocyte hypertrophy parallels alterations of mitochondrial status in a cell model for adipose tissue dysfunction in obesity

Francesca Baldini; Rita Fabbri; Carola Eberhagen; Adriana Voci; Piero Portincasa; Hans Zischka; Laura Vergani

doi:10.1016/j.lfs.2020.118812

Adipocyte hypertrophy parallels alterations of mitochondrial status in a cell model for adipose tissue dysfunction in obesity

Life Sci. 2021 Jan 15:265:118812. doi: 10.1016/j.lfs.2020.118812. Epub 2020 Dec 2.

Authors

Francesca Baldini¹, Rita Fabbri², Carola Eberhagen³, Adriana Voci², Piero Portincasa⁴, Hans Zischka⁵, Laura Vergani⁶

Affiliations

¹ Department of Experimental Medicine (DIMES), University of Genova, Genova, Italy.
² Department of Earth, Environment and Life Sciences (DISTAV), University of Genova, Corso Europa 26, 16132 Genova, Italy.
³ Institute of Molecular Toxicology and Pharmacology, Helmholtz Center Munich, German Research Center for Environmental Health, Neuherberg, Germany.
⁴ Division of Internal Medicine, Department of Biomedical Sciences and Human Oncology, University School of Medicine, 70124 Bari, Italy.
⁵ Institute of Molecular Toxicology and Pharmacology, Helmholtz Center Munich, German Research Center for Environmental Health, Neuherberg, Germany; Institute of Toxicology and Environmental Hygiene, Technical University of Munich, School of Medicine, Munich, Germany.
⁶ Department of Earth, Environment and Life Sciences (DISTAV), University of Genova, Corso Europa 26, 16132 Genova, Italy. Electronic address: laura.vergani@unige.it.

PMID: 33278396
DOI: 10.1016/j.lfs.2020.118812

Abstract

Aims: Adipocyte hypertrophy is the main cause of obesity. A deeper understanding of the molecular mechanisms regulating adipocyte dysfunction may help to plan strategies to treat/prevent obesity and its metabolic complications. Here, we investigated in vitro the molecular alterations associated with early adipocyte hypertrophy, focusing on mitochondrial dysfunction.

Main methods: As model of adipocyte hypertrophy, we employed 3T3-L1 preadipocytes firstly differentiated into mature adipocytes, then cultured with long-chain fatty acids. As a function of differentiation and hypertrophy, we assessed triglyceride content, lipid droplet size, radical homeostasis by spectrophotometry and microscopy, as well as the expression of PPARγ, adiponectin and metallothioneins. Mitochondrial status was investigated by electron microscopy, oxygraph 2 k (O2K) high-resolution respirometry, fluorimetry and western blot.

Key findings: Compared to mature adipocytes, hypertrophic adipocytes showed increased triglyceride accumulation and lipid peroxidation, larger or unique lipid droplet, up-regulated expression of PPARγ, adiponectin and metallothioneins. At mitochondrial level, early-hypertrophic adipocytes exhibited: (i) impaired mitochondrial oxygen consumption with parallel reduction in the mitochondrial complexes; (ii) no changes in citrate synthase and HSP60 expression, and in the inner mitochondrial membrane polarization; (iii) no stimulation of mitochondrial fatty acid oxidation. Our findings indicate that the content, integrity, and catabolic activity of mitochondria were rather unchanged in early hypertrophic adipocytes, while oxygen consumption and oxidant production were altered.

Significance: In the model of early adipocyte hypertrophy exacerbated oxidative stress and impaired mitochondrial respiration were observed, likely depending on reduction in the mitochondrial complexes, without changes in mitochondrial mass and integrity.

Keywords: Adipocyte hypertrophy; Mitochondria; Mitochondrial respiration; Obesity; Oxidative stress.

MeSH terms

3T3-L1 Cells
Adipocytes / pathology*
Adipose Tissue / pathology*
Animals
Cell Differentiation
Electron Transport / physiology
Hypertrophy
Mice
Mitochondria / pathology*
Obesity / physiopathology*
Oxidative Stress / physiology
Oxygen Consumption / physiology