Abstract

Mg2+ is an abundant intracellular cation that is critical for the control of a wide array of intracellular processes. However, relatively little is known about the homeostatic mechanisms that control intracellular free Mg2+ ([Mg2+]i, nor about mechanisms that might perturb (Mg2+]i. It has recently been shown that stimuli that are normally considered excitotoxic to neurons produce millimolar increases in [Mg2+]i in cultured neurons. The long term goal of this project is to understand the role of [Mg2+]i in processes associated with neuronal injury and to develop effective treatment strategies based on manipulation of Mg2+ homeostasis. This will be accomplished by the following specific aims: 1. characterization of mechanisms that alter [Mg2+]i. [Mg2+]i will be measured in cultured rat forebrain neurons using Mg2+-sensitive fluorescent dyes. The characteristics of the (Mg2+]i response to glutamate receptor activation will be established, and the hypothesis that the [Mg2+]i is proportional to Ca2+ will be tested. Fluorescence imaging techniques will be used to determine the source of the intracellular Mg2+ release. 2. Elucidation of the mechanisms of [Mg2+]i homeostasis. The role of a number of putative cellular Mg2+ buffering mechanisms will be established. In particular, the hypothesis that Na+/Mg2+ exchange contributes to neuronal Mg2+ buffering will be examined. 3. Determination of the role of changes in intracellular Mg2+ in excitotoxicity. Preliminary results show that excitotoxic stimuli are very effective at raising [Mg2+]i. The role of elevated [Mg2+]i as well as the effect of tissue Mg2+ loss in excitotoxicity will be investigated. This will establish the role of intracellular Mg2+ in excitotoxic cell death and highlight novel therapeutic approaches to ameliorating neuronal injury. 4. Regulation of neuronal Ca2+ homeostasis by intracellular Mg2+. There is very little information available about the role of intracellular Mg2+ in regulating neuronal function. The influence of [Mg2+]i changes on Ca2+ entry and Ca2+ homeostasis will be investigated, and will provide another link between [Mg2+]i changes and excitotoxicity. These studies will provide substantial new information about the role of a poorly understood cation in the regulation of neuronal function. More importantly, these studies will reveal the involvement of Mg2+ in excitotoxic neuronal injury and thereby highlight mechanism that contribute to neuronal death. We also anticipate that these studies will generate novel concepts about the treatment of neuronal injury based on manipulation of the Mg2+ environment and thereby positively impact the treatment of stroke and traumatic brain injury.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS034138-03
Application #
2416386
Study Section
Neurological Sciences Subcommittee 1 (NLS)
Program Officer
Cheung, Mary Ellen
Project Start
1995-05-01
Project End
1999-04-30
Budget Start
1997-05-01
Budget End
1998-04-30
Support Year
3
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
University of Pittsburgh
Department
Pharmacology
Type
Schools of Medicine
DUNS #
053785812
City
Pittsburgh
State
PA
Country
United States
Zip Code
15213

  Publications

Devinney, Michael J; Malaiyandi, Latha M; Vergun, Olga et al. (2009) A comparison of Zn2+- and Ca2+-triggered depolarization of liver mitochondria reveals no evidence of Zn2+-induced permeability transition. Cell Calcium 45:447-55
Dineley, Kirk E; Devinney 2nd, Michael J; Zeak, Jennifer A et al. (2008) Glutamate mobilizes [Zn2+] through Ca2+ -dependent reactive oxygen species accumulation. J Neurochem 106:2184-93
Malaiyandi, Latha M; Vergun, Olga; Dineley, Kirk E et al. (2005) Direct visualization of mitochondrial zinc accumulation reveals uniporter-dependent and -independent transport mechanisms. J Neurochem 93:1242-50
Malaiyandi, Latha M; Honick, Anthony S; Rintoul, Gordon L et al. (2005) Zn2+ inhibits mitochondrial movement in neurons by phosphatidylinositol 3-kinase activation. J Neurosci 25:9507-14
Devinney 2nd, Michael J; Reynolds, Ian J; Dineley, Kirk E (2005) Simultaneous detection of intracellular free calcium and zinc using fura-2FF and FluoZin-3. Cell Calcium 37:225-32
Dineley, Kirk E; Richards, Lauren L; Votyakova, Tatyana V et al. (2005) Zinc causes loss of membrane potential and elevates reactive oxygen species in rat brain mitochondria. Mitochondrion 5:55-65
Malaiyandi, Latha M; Dineley, Kirk E; Reynolds, Ian J (2004) Divergent consequences arise from metallothionein overexpression in astrocytes: zinc buffering and oxidant-induced zinc release. Glia 45:346-53
Dineley, Kirk E; Votyakova, Tatyana V; Reynolds, Ian J (2003) Zinc inhibition of cellular energy production: implications for mitochondria and neurodegeneration. J Neurochem 85:563-70
Dineley, K E; Brocard, J B; Reynolds, I J (2002) Elevated intracellular zinc and altered proton homeostasis in forebrain neurons. Neuroscience 114:439-49
Kress, Geraldine J; Dineley, Kirk E; Reynolds, Ian J (2002) The relationship between intracellular free iron and cell injury in cultured neurons, astrocytes, and oligodendrocytes. J Neurosci 22:5848-55

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