Muller 2013 Exp Neurol: Difference between revisions

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{{Publication
{{Publication
|title=Muller AP, Haas CB, Camacho-Pereira J, Brochier AW, Gnoatto J, Zimmer ER, de Souza DO, Galina A, Portela LV (2013) Insulin prevents mitochondrial generation of H2O2 in rat brain. Exp Neurol 247:66-72. Β 
|title=Muller AP, Haas CB, Camacho-Pereira J, Brochier AW, Gnoatto J, Zimmer ER, de Souza DO, Galina A, Portela LV (2013) Insulin prevents mitochondrial generation of H2O2 in rat brain. Exp Neurol 247:66-72.
|info=[http://www.ncbi.nlm.nih.gov/pubmed/23499835 PMID: 23499835]
|info=[http://www.ncbi.nlm.nih.gov/pubmed/23499835 PMID: 23499835]
|authors=Muller AP, Haas CB, Camacho-Pereira J, Brochier AW, Gnoatto J, Zimmer ER, de Souza DO, Galina A, Portela LV
|authors=Muller AP, Haas CB, Camacho-Pereira J, Brochier AW, Gnoatto J, Zimmer ER, de Souza DO, Galina A, Portela LV
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{{Labeling
{{Labeling
|instruments=Oxygraph-2k
|area=Respiration, mt-Medicine
|additional=Labels
|organism=Rat
|tissues=Nervous system
|couplingstates=LEAK, OXPHOS, ETS
|substratestates=CI, CII
|instruments=Oxygraph-2k, Fluorometry
}}
}}

Revision as of 13:16, 15 January 2014

Publications in the MiPMap
Muller AP, Haas CB, Camacho-Pereira J, Brochier AW, Gnoatto J, Zimmer ER, de Souza DO, Galina A, Portela LV (2013) Insulin prevents mitochondrial generation of H2O2 in rat brain. Exp Neurol 247:66-72.

Β» PMID: 23499835

Muller AP, Haas CB, Camacho-Pereira J, Brochier AW, Gnoatto J, Zimmer ER, de Souza DO, Galina A, Portela LV (2013) Exp Neurol

Abstract: The mitochondrial electron transport system (ETS) is a main source of cellular ROS, including hydrogen peroxide (Hβ‚‚Oβ‚‚). The production of Hβ‚‚Oβ‚‚ also involves the mitochondrial membrane potential (ΔΨm) and oxygen consumption. Impaired insulin signaling causes oxidative neuronal damage and places the brain at risk of neurodegeneration. We evaluated whether insulin signaling cross-talks with ETS components (complexes I and Fβ‚€F₁ATP synthase) and ΔΨm to regulate mitochondrial Hβ‚‚Oβ‚‚ production, in tissue preparations from rat brain. Insulin (50 to 100 ng/mL) decreased Hβ‚‚Oβ‚‚ production in synaptosomal preparations in high Na(+) buffer (polarized state), stimulated by glucose and pyruvate, without affecting the oxygen consumption. In addition, insulin (10 to 100 ng/mL) decreased Hβ‚‚Oβ‚‚ production induced by succinate in synaptosomes in high K(+) (depolarized state), whereas wortmannin and LY290042, inhibitors of the PI3K pathway, reversed this effect; heated insulin had no effect. Insulin decreased Hβ‚‚Oβ‚‚ production when complexes I and Fβ‚€F₁ATP synthase were inhibited by rotenone and oligomycin respectively suggesting a target effect on complex III. Also, insulin prevented the generation of maximum level of βˆ†Ξ¨m induced by succinate. The PI3K inhibitors and heated insulin maintained the maximum level of βˆ†Ξ¨m induced by succinate in synaptosomes in a depolarized state. Similarly, insulin decreased ROS production in neuronal cultures. In mitochondrial preparations, insulin neither modulated H2O2 production or oxygen consumption. In conclusion, the normal downstream insulin receptor signaling is necessary to regulate complex III of ETS avoiding the generation of maximal βˆ†Ξ¨m and increased mitochondrial H2O2 production. β€’ Keywords: Brain metabolism, H(2)O(2) production, Insulin signaling, Mitochondria

β€’ O2k-Network Lab: BR Rio de Janeiro Galina A, BR Rio de Janeiro Institute Biomedical Chemistry


Labels: MiParea: Respiration, mt-Medicine 


Organism: Rat  Tissue;cell: Nervous system 


Coupling state: LEAK, OXPHOS, ETS"ETS" is not in the list (LEAK, ROUTINE, OXPHOS, ET) of allowed values for the "Coupling states" property. 

HRR: Oxygraph-2k, Fluorometry"Fluorometry" is not in the list (Oxygraph-2k, TIP2k, O2k-Fluorometer, pH, NO, TPP, Ca, O2k-Spectrophotometer, O2k-Manual, O2k-Protocol, ...) of allowed values for the "Instrument and method" property. 


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