PPARγ is a major regulator of branched-chain amino acid blood levels and catabolism in white and brown adipose tissues.

dc.contributor.authorBlanchard, Pierre-Gilles
dc.contributor.authorMoreira, Rafael Junges
dc.contributor.authorCastro, Érique de
dc.contributor.authorCaron, Alexandre
dc.contributor.authorCôté, Marie
dc.contributor.authorAndrade, Maynara Lucca
dc.contributor.authorSilva, Tiago Eugênio Oliveira da
dc.contributor.authorSilva, Milene Ortiz
dc.contributor.authorPeixoto, Álbert Souza
dc.contributor.authorRuas, France Anne Dias
dc.contributor.authorGélinas, Yves
dc.contributor.authorCota, Renata Guerra de Sá
dc.contributor.authorDeshaies, Yves
dc.contributor.authorFestuccia, William Tadeu Lara
dc.date.accessioned2019-04-09T15:17:14Z
dc.date.available2019-04-09T15:17:14Z
dc.date.issued2018
dc.description.abstractObjective We investigated whether PPARγ modulates adipose tissue BCAA metabolism, and whether this mediates the attenuation of obesity-associated insulin resistance induced by pharmacological PPARγ activation. Methods Mice with adipocyte deletion of one or two PPARγ copies fed a chow diet and rats fed either chow, or high fat (HF) or HF supplemented with BCAA (HF/BCAA) diets treated with rosiglitazone (30 or 15 mg/kg/day, 14 days) were evaluated for glucose and BCAA homeostasis. Results Adipocyte deletion of one PPARγ copy increased mice serum BCAA and reduced inguinal white (iWAT) and brown (BAT) adipose tissue BCAA incorporation into triacylglycerol, as well as mRNA levels of branched-chain aminotransferase (BCAT)2 and branched-chain α-ketoacid dehydrogenase (BCKDH) complex subunits. Adipocyte deletion of two PPARγ copies induced lipodystrophy, severe glucose intolerance and markedly increased serum BCAA. Rosiglitazone abolished the increase in serum BCAA induced by adipocyte PPARγ deletion. In rats, HF increased serum BCAA, such levels being further increased by BCAA supplementation. Rosiglitazone, independently of diet, lowered serum BCAA and upregulated iWAT and BAT BCAT and BCKDH activities. This was associated with a reduction in mTORC1-dependent inhibitory serine phosphorylation of IRS1 in skeletal muscle and whole-body insulin resistance evaluated by HOMA-IR. Conclusions PPARγ, through the regulation of both BAT and iWAT BCAA catabolism in lipoeutrophic mice and muscle insulin responsiveness and proteolysis in lipodystrophic mice, is a major determinant of circulating BCAA levels. PPARγ agonism, therefore, may improve whole-body and muscle insulin sensitivity by reducing blood BCAA, alleviating mTORC1-mediated inhibitory IRS1 phosphorylation.pt_BR
dc.identifier.citationBLANCHARD, P. G. et al. PPARγ is a major regulator of branched-chain amino acid blood levels and catabolism in white and brown adipose tissues. Metabolism, v. 89, p. 27-38, dez. 2018. Disponível em: <https://www.sciencedirect.com/science/article/pii/S0026049518302117?via%3Dihub>. Acesso em: 25 fev. 2019.pt_BR
dc.identifier.issn00260495
dc.identifier.urihttp://www.repositorio.ufop.br/handle/123456789/10985
dc.identifier.uri2https://www.sciencedirect.com/science/article/pii/S0026049518302117pt_BR
dc.language.isoen_USpt_BR
dc.rightsrestritopt_BR
dc.titlePPARγ is a major regulator of branched-chain amino acid blood levels and catabolism in white and brown adipose tissues.pt_BR
dc.typeArtigo publicado em periodicopt_BR

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