Abstract

This project seeks to identify the cellular mechanisms that regulate neurite outgrowth and synapse replacement in the striatum (ST) in response to injury and the effect of aging on these processes. Studies conducted during the previous funding period support the belief that the cellular basis of reactive synaptogenesis involves the activation of specific sets of partially overlapping developmental signals that are cell type, brain region and lesion specific, and that these responses may be differentially affected by age. However, while previous anatomical studies have readily demonstrated the ability of neurons to form new synaptic circuits in response to brain injury the cellular mechanisms that regulate reactive synaptogenesis remain unclear. The studies proposed are a direct extension of the work completed previously and will test four general hypotheses: 1) that different sets of growth associated proteins regulate neurite outgrowth in corticostriatal neurons in response to different deafferentation lesions: 2) that the time course for debris removal, terminal proliferation and synapse replacement in the ST after injury is influenced by age and the type of lesion involved; 3) that the new pattern of synaptic innervation that is formed in the ST is different after lesions of the cortex, substantia nigra or both, and are reflected in the pharmacological properties of the synaptic input on striatal neurons; and 4) that chronic dietary restriction or treatment with the dopamine agonist pergolide to manipulate the effects of aging in the ST (i.e., reactive astrocytosis, loss of D2 receptors) will reverse the effects of aging on dendrite remodeling and neurite outgrowth found after the cortex lesion. We will use experimental deafferentation lesions in young (4 mos) and old (24 mos) rats to model different combinations of neurotransmitter deficits that may effect neurite outgrowth and synapse replacement in the ST following brain injury. In addition, we will screen aged rats prior to surgery, using the balance beam test, to identify subsets of old rats with nigrostriatal deficits that may alter their ability to respond to the lesion. We will also assess the rate of functional recovery to correlate with our morphological and molecular data. Morphological remodeling of afferent input to the ST will be evaluated using ultrastructural methods; while synaptic physiology of the anatomically reorganized ST will be examined by electrophysiological analysis. In addition, we will use in in situ hybridization and western blot methods to define the time course of changes in the levels of mRNAs and proteins that we hypothesize are associated with the promotion of neurite outgrowth and synapse replacement in the ST (i.e., SCG-10, GAP-43, BDNF, GDNF, etc.).

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute on Aging (NIA)
Type
Research Program Projects (P01)
Project #
5P01AG009793-09
Application #
6098300
Study Section
Project Start
1999-06-15
Project End
2000-05-31
Budget Start
1998-10-01
Budget End
1999-09-30
Support Year
9
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
University of Southern California
Department
Type
DUNS #
041544081
City
Los Angeles
State
CA
Country
United States
Zip Code
90089

  Publications

Chinta, S J; Lieu, C A; Demaria, M et al. (2013) Environmental stress, ageing and glial cell senescence: a novel mechanistic link to Parkinson's disease? J Intern Med 273:429-36
Vali, Shireen; Chinta, Shankar J; Peng, Jun et al. (2008) Insights into the effects of alpha-synuclein expression and proteasome inhibition on glutathione metabolism through a dynamic in silico model of Parkinson's disease: validation by cell culture data. Free Radic Biol Med 45:1290-301
Jakowec, Michael W; Nixon, Kerry; Hogg, Elizabeth et al. (2004) Tyrosine hydroxylase and dopamine transporter expression following 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine-induced neurodegeneration of the mouse nigrostriatal pathway. J Neurosci Res 76:539-50
Finch, Caleb E (2003) Neurons, glia, and plasticity in normal brain aging. Neurobiol Aging 24 Suppl 1:S123-7; discussion S131
McNeill, Thomas H; Brown, Sally A; Hogg, Elizabeth et al. (2003) Synapse replacement in the striatum of the adult rat following unilateral cortex ablation. J Comp Neurol 467:32-43
Robinson, Siobhan; Freeman, Pierre; Moore, Cynthia et al. (2003) Acute and subchronic MPTP administration differentially affects striatal glutamate synaptic function. Exp Neurol 180:74-87
Jha, Nandita; Kumar, M Jyothi; Boonplueang, Rapee et al. (2002) Glutathione decreases in dopaminergic PC12 cells interfere with the ubiquitin protein degradation pathway: relevance for Parkinson's disease? J Neurochem 80:555-61
Rozovsky, Irina; Hoving, Saske; Anderson, Christopher P et al. (2002) Equine estrogens induce apolipoprotein E and glial fibrillary acidic protein in mixed glial cultures. Neurosci Lett 323:191-4
Finch, C E (2002) Neurons, glia, and plasticity in normal brain aging. Adv Gerontol 10:35-9
Jiang, D; Jha, N; Boonplueang, R et al. (2001) Caspase 3 inhibition attenuates hydrogen peroxide-induced DNA fragmentation but not cell death in neuronal PC12 cells. J Neurochem 76:1745-55

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