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Selective Oestrogen Receptor Modulators Differentially Potentiate Brain Mitochondrial Function
Author(s) -
Irwin R. W.,
Yao J.,
To J.,
Hamilton R. T.,
Cadenas E.,
Brinton R. D.
Publication year - 2012
Publication title -
journal of neuroendocrinology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.062
H-Index - 116
eISSN - 1365-2826
pISSN - 0953-8194
DOI - 10.1111/j.1365-2826.2011.02251.x
Subject(s) - medicine , endocrinology , biology , mitochondrion , bioenergetics , estrogen receptor , agonist , receptor , microbiology and biotechnology , cancer , breast cancer
The mitochondrial energy‐transducing capacity of the brain is important for long‐term neurological health and is influenced by endocrine hormone responsiveness. The present study aimed to determine the role of oestrogen receptor (ER) subtypes in regulating mitochondrial function using selective agonists for ERα (propylpyrazoletriol; PPT) and ERβ (diarylpropionitrile; DPN). Ovariectomised female rats were treated with 17β‐oestradiol (E 2 ), PPT, DPN or vehicle control. Both ER selective agonists significantly increased the mitochondrial respiratory control ratio and cytochrome oxidase (COX) activity relative to vehicle. Western blots of purified whole brain mitochondria detected ERα and, to a greater extent, ERβ localisation. Pre‐treatment with DPN, an ERβ agonist, significantly increased ERβ association with mitochondria. In the hippocampus, DPN activated mitochondrial DNA‐encoded COX I expression, whereas PPT was ineffective, indicating that mechanistically ERβ, and not ERα, activated mitochondrial transcriptional machinery. Both selective ER agonists increased protein expression of nuclear DNA‐encoded COX IV, suggesting that activation of ERβ or ERα is sufficient. Selective ER agonists up‐regulated a panel of bioenergetic enzymes and antioxidant defence proteins. Up‐regulated proteins included pyruvate dehydrogenase, ATP synthase, manganese superoxide dismutase and peroxiredoxin V. In vitro , whole cell metabolism was assessed in live primary cultured hippocampal neurones and mixed glia. The results of analyses conducted in vitro were consistent with data obtained in vivo . Furthermore, lipid peroxides, accumulated as a result of hormone deprivation, were significantly reduced by E 2 , PPT and DPN. These findings suggest that the activation of both ERα and ERβ is differentially required to potentiate mitochondrial function in brain. As active components in hormone therapy, synthetically designed oestrogens as well as natural phyto‐oestrogen cocktails can be tailored to improve brain mitochondrial endpoints.