Literature DB >> 15950756

Modulatory effect of glutathione status and antioxidants on methylmercury-induced free radical formation in primary cultures of cerebral astrocytes.

Gouri Shanker1, Tore Syversen, Judy L Aschner, Michael Aschner.   

Abstract

Excessive free radical formation has been implicated as one of the causative factors in neurotoxic damage associated with variety of metals, including methylmercury (MeHg). Although the mechanism(s) associated with MeHg-dependent neurotoxicity remains far from clear, overwhelming data give credence to a mediatory role for astrocytes, a major cell type that preferentially accumulates MeHg. To extend our recent findings of MeHg-induced increase in ROS formation (G. Shanker, J.L. Aschner, T. Syversen et al., Free radical formation in cerebral cortical astrocytes in culture induced by methylmercury, Mol. Brain Res. 128 (2004) 48-57), the present studies were designed to assess the effect of modulating intracellular glutathione (GSH) content, on ROS generation, in the absence and presence of MeHg. Intracellular GSH was reduced by treatment with 100 microM buthionine-L-sulfoxane (BSO) for 24 h, and increased by treatment with 1 mM l-2-oxothiazolidine-4-carboxylic acid (OTC) for 24 h. Additionally, the effects of the selective antioxidants, catalase (1000 U/ml for 1 h), an H2O2 scavenger, and n-propyl gallate (100 microM for 1 h), a superoxide radical (*O2-) and possibly hydroxyl radical (*OH) scavenger on MeHg-induced ROS formation were examined. After these treatments, astrocytes were exposed to +/-10 microM MeHg for 30 min, following which the fluorescent probes, CM-H2DCFA and CM-H2XRos were added; 20 min later, laser scanning confocal microscopy (LSCM) images were obtained. Exposure of astrocytes for 24 h to 100 microM BSO, a GSH synthesis inhibitor, led to a significant increase in mitochondrial ROS (i.e., *O2-, *NO, and ONOO-) formation, as assessed with CM-H2XRos mitotracker red dye. Similarly, BSO increased ROS formation in various intracellular organelles, as assessed with CM-H2DCFDA. BSO in combination with MeHg increased fluorescence levels in astrocytes to levels above those noted with BSO or MeHg alone, but this effect was statistically indistinguishable from either of these groups (BSO or MeHg). Pretreatment of astrocytes for 24 h with 1 mM OTC abolished the MeHg-induced increase in ROS. Results similar to those obtained with OTC were observed with the free radical scavenger, n-propyl gallate (n-PG). The latter had no significant effects on astrocytic fluorescence when administered alone. This *O2- and possibly *OH radical scavenger significantly attenuated MeHg-induced ROS formation. Catalase, an H2O2 scavenger, was less effective in reducing MeHg-induced ROS formation. Taken together, these studies point to the important protective effect of adequate intracellular GSH content as well as antioxidants against MeHg-triggered oxidative stress in primary astrocyte cultures.

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Year:  2005        PMID: 15950756     DOI: 10.1016/j.molbrainres.2005.02.006

Source DB:  PubMed          Journal:  Brain Res Mol Brain Res        ISSN: 0169-328X


  36 in total

Review 1.  Neurobehavioural and molecular changes induced by methylmercury exposure during development.

Authors:  Carolina Johansson; Anna F Castoldi; Natalia Onishchenko; Luigi Manzo; Marie Vahter; Sandra Ceccatelli
Journal:  Neurotox Res       Date:  2007-04       Impact factor: 3.911

2.  Comparison of alterations in amino acids content in cultured astrocytes or neurons exposed to methylmercury separately or in co-culture.

Authors:  Zhaobao Yin; Jan Albrecht; Tore Syversen; Haiyan Jiang; Marshall Summar; Joao B T Rocha; Marcelo Farina; Michael Aschner
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Review 3.  The Putative Role of Environmental Mercury in the Pathogenesis and Pathophysiology of Autism Spectrum Disorders and Subtypes.

Authors:  G Morris; B K Puri; R E Frye; M Maes
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Review 4.  Human-induced pluripotent stems cells as a model to dissect the selective neurotoxicity of methylmercury.

Authors:  Lisa M Prince; Michael Aschner; Aaron B Bowman
Journal:  Biochim Biophys Acta Gen Subj       Date:  2019-02-10       Impact factor: 3.770

5.  Role of oxidative stress and the mitochondrial permeability transition in methylmercury cytotoxicity.

Authors:  Marianne Polunas; Alycia Halladay; Ronald B Tjalkens; Martin A Philbert; Herbert Lowndes; Kenneth Reuhl
Journal:  Neurotoxicology       Date:  2011-08-19       Impact factor: 4.294

6.  Structure-activity relationship of flavonoids derived from medicinal plants in preventing methylmercury-induced mitochondrial dysfunction.

Authors:  Jeferson L Franco; Thais Posser; Fabiana Missau; Moacir G Pizzolatti; Adair R S Dos Santos; Diogo O Souza; Michael Aschner; João B T Rocha; Alcir L Dafre; Marcelo Farina
Journal:  Environ Toxicol Pharmacol       Date:  2010-11-01       Impact factor: 4.860

7.  Protective effect of a novel peptide against methylmercury-induced toxicity in rat primary astrocytes.

Authors:  Uri Wormser; Berta Brodsky; Dejan Milatovic; Yoram Finkelstein; Marcelo Farina; Joao B Rocha; Michael Aschner
Journal:  Neurotoxicology       Date:  2011-12-14       Impact factor: 4.294

8.  Common effects of lithium and valproate on mitochondrial functions: protection against methamphetamine-induced mitochondrial damage.

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Journal:  Int J Neuropsychopharmacol       Date:  2009-01-19       Impact factor: 5.176

9.  Prenatal methylmercury exposure hampers glutathione antioxidant system ontogenesis and causes long-lasting oxidative stress in the mouse brain.

Authors:  James Stringari; Adriana K C Nunes; Jeferson L Franco; Denise Bohrer; Solange C Garcia; Alcir L Dafre; Dejan Milatovic; Diogo O Souza; João B T Rocha; Michael Aschner; Marcelo Farina
Journal:  Toxicol Appl Pharmacol       Date:  2007-10-22       Impact factor: 4.219

10.  Effect of garlic on isoniazid and rifampicin-induced hepatic injury in rats.

Authors:  Ravinder Pal; Kim Vaiphei; Arbab Sikander; Kartar Singh; Satya V Rana
Journal:  World J Gastroenterol       Date:  2006-01-28       Impact factor: 5.742

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