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Anatomical distribution of primary amine oxidase activity in four adipose depots and plasma of severely obese women with or without a dysmetabolic profile
Authors:Christian Carpéné  Francisco Les  Mounia Hasnaoui  Simon Biron  Picard Marceau  Denis Richard  Jean Galitzky  Denis R Joanisse  Pascale Mauriège
Institution:1.INSERM U 1048, Institut des Maladies Métaboliques et Cardiovasculaires, Institut National de la Santé et de la Recherche Médicale (INSERM U1048) and Université Paul Sabatier (I2MC-UPS) Toulouse,Toulouse,France;2.Department of Pharmacology,University San Jorge,Zaragoza,Spain;3.Department of Surgery, Faculty of Medicine, Centre de Recherche de l’Institut Universitaire de Cardiologie et de Pneumologie de Québec,Université Laval,Québec,Canada;4.Department of Physiology, Faculty of Medicine, Centre de Recherche de l’Institut Universitaire de Cardiologie et de Pneumologie de Québec,Université Laval,Québec,Canada;5.Department of Kinesiology, Faculty of Medicine, Centre de Recherche de l’Institut Universitaire de Cardiologie et de Pneumologie de Québec,Université Laval,Québec,Canada;6.Department of Kinesiology,Laval University,Québec,Canada
Abstract:Semicarbazide-sensitive amine oxidase (SSAO), identical to primary amine oxidase or vascular adhesion protein-1, is a membrane enzyme that generates hydrogen peroxide. SSAO is highly expressed at the adipocyte surface, and its plasma levels increase with type 2 diabetes. Since visceral adipose tissue (AT) is more tightly associated with obesity complications than subcutaneous (SC) abdominal fat, we compared SSAO activity in plasma and 4 distinct AT locations in 48 severely obese women (body mass index (BMI), averaging 54 ± 11 kg/m2), with or without a dysmetabolic profile. Higher glucose and triacylglycerol levels vs lower high-density lipoprotein (HDL)-cholesterol characterized dysmetabolic women (DYS; n = 25) from non-dysmetabolic (NDYS; n = 23), age- and weight-matched subjects. SC, mesenteric (ME), omental (OM), and round ligament (RL) fat locations were collected during bariatric surgery. SSAO capacity to oxidize up to 1 mM benzylamine was determined in AT and plasma with radiometric and fluorimetric methods. Plasma SSAO was higher in the DYS group. SSAO activity was higher in fat than in plasma, when expressed as radiolabeled benzaldehyde per milligram of protein. In ATs from DYS women, protein content was 10 % higher, and basal hydrogen peroxide release lower than in NDYS subjects, except for RL location. The SSAO affinity towards benzylamine did not exhibit regional variation and was not altered by a dysmetabolic profile (K m averaging 184 ± 7 μM; n = 183). Although radiometric and fluorimetric methods gave different estimates of oxidase activity, both indicated that AT SSAO activity did not vary according to anatomical location and/or metabolic status in severely obese women.
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