Abstract

The goal of the work proposed in this application is to decrease fat stores by increasing oxidation. The hypothesis underlying this approach is that preventing inhibition of respiration induced by ROS will lead to increased oxidation and decreased fat storage. Adipocyte respiration above basal is inhibited. However, scavengers of reactive oxygen species (ROS), pyruvate or N-acetyl cysteine, can restore O2 consumption in rat adipocytes and decrease fat stores in human adipocytes. This was observed only in intact cells and not in isolated mitochondria suggesting that ROS production required the high fat environment of the intact cell. We have developed a novel long-lasting preparation of immobilized cultured adipocytes that permits repeated measurement of O2 consumption and image analysis of fluorescent molecules. To test our hypothesis we will use isolated rat adipocytes and mitochondria and differentiated human preadipocytes to perform the following Aims:
Aim 1 is to determine if ROS removal stimulates respiration and decreases TG stores in rat and human adipocytes. The prediction will be tested that there is a relationship between ROS and TG stores such that decreasing ROS through over-expression of superoxide dismutase, peroxiredoxin or glutathione peroxidase will decrease TG stores. We will simultaneously measure mitochondrial membrane potential (??) and respiration to assess coupling.
Aim 2 is to identify the site in the respiratory chain that is inhibited by ROS. To learn the identity of the site, we will measure O2 consumption in adipocytes from substrates that enter the respiratory chain through Complexes I, III or IV. Relief of inhibition will be indicated by increased respiration.
Aim 3 is to determine whether O2-, H2O2, NO or other ROS mediate inhibited respiration. Using submitochondrial particles derived from adipocytes we will identify the inhibitory ROS species and their specific site of action. Flux will be measured in the presence of ROS and site-specific substrates.
Aim 4 will determine the mechanism of low adipocyte apoptosis and turnover amid evidence of strong ROS action in mitochondria. We will map mitochondrial networking in adipocytes using photoactivation and test the effect of network alteration through gene knockdown. We anticipate that uncoupling between ROS and apoptosis is an essential component of adipocyte FFA handling. The anticipated outcome of these experiments is identification of the mechanism responsible for the unique inhibition of adipocyte respiration by ROS and ways to overcome this inhibition. Respiration in adipocytes has been little investigated, due in part, to the misconception that it is not important. These experiments could reverse the thrifty phenotype and possibly lend insight into the thrifty genotype and its role in the development of obesity. ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK056690-07
Application #
7194284
Study Section
Special Emphasis Panel (ZRG1-EMNR-B (90))
Program Officer
Haft, Carol R
Project Start
1999-12-01
Project End
2011-01-31
Budget Start
2007-02-01
Budget End
2008-01-31
Support Year
7
Fiscal Year
2007
Total Cost
$364,106
Indirect Cost

  Institution

Name
Boston Medical Center
Department
Type
DUNS #
005492160
City
Boston
State
MA
Country
United States
Zip Code
02118

  Publications

Benador, Ilan Y; Veliova, Michaela; Mahdaviani, Kiana et al. (2018) Mitochondria Bound to Lipid Droplets Have Unique Bioenergetics, Composition, and Dynamics that Support Lipid Droplet Expansion. Cell Metab 27:869-885.e6
Mahdaviani, Kiana; Benador, Ilan Y; Su, Shi et al. (2017) Mfn2 deletion in brown adipose tissue protects from insulin resistance and impairs thermogenesis. EMBO Rep 18:1123-1138
Schwartz, Stanley S; Epstein, Solomon; Corkey, Barbara E et al. (2016) The Time Is Right for a New Classification System for Diabetes: Rationale and Implications of the ?-Cell-Centric Classification Schema. Diabetes Care 39:179-86
Trudeau, Kyle M; Colby, Aaron H; Zeng, Jialiu et al. (2016) Lysosome acidification by photoactivated nanoparticles restores autophagy under lipotoxicity. J Cell Biol 214:25-34
Cerqueira, Fernanda M; Chausse, Bruno; Baranovski, Boris M et al. (2016) Diluted serum from calorie-restricted animals promotes mitochondrial ?-cell adaptations and protect against glucolipotoxicity. FEBS J 283:822-33
Forni, Maria Fernanda; Peloggia, Julia; Trudeau, Kyle et al. (2016) Murine Mesenchymal Stem Cell Commitment to Differentiation Is Regulated by Mitochondrial Dynamics. Stem Cells 34:743-55
Nocito, Laura; Kleckner, Amber S; Yoo, Elsia J et al. (2015) The extracellular redox state modulates mitochondrial function, gluconeogenesis, and glycogen synthesis in murine hepatocytes. PLoS One 10:e0122818
Wikstrom, Jakob D; Mahdaviani, Kiana; Liesa, Marc et al. (2014) Hormone-induced mitochondrial fission is utilized by brown adipocytes as an amplification pathway for energy expenditure. EMBO J 33:418-36
Simmons, Amber L; Schlezinger, Jennifer J; Corkey, Barbara E (2014) What Are We Putting in Our Food That Is Making Us Fat? Food Additives, Contaminants, and Other Putative Contributors to Obesity. Curr Obes Rep 3:273-85
Las, Guy; Shirihai, Orian S (2014) Miro1: new wheels for transferring mitochondria. EMBO J 33:939-41

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