4.5 Article

Differential ultrastructural alterations in the Vglut2 glutamatergic input to the substantia nigra pars compacta/pars reticulata following nigrostriatal dopamine loss in a progressive mouse model of Parkinson's disease

Journal

EUROPEAN JOURNAL OF NEUROSCIENCE
Volume 53, Issue 7, Pages 2061-2077

Publisher

WILEY
DOI: 10.1111/ejn.14894

Keywords

electron microscopy; immunohistochemistry; MPTP; subthalamic nucleus; vesicular glutamate transporter 2

Categories

Funding

  1. Department of Veterans' Affairs, United States [I01 BX000552, I01 BX001643]
  2. Research and Development
  3. U.S. Department of Veterans Affairs

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The study found that there are differential changes in glutamate release from Vglut2+ nerve terminals synapsing within the substantia nigra pars compacta (SNpc) and pars reticulata (SNpr) following dopamine loss in Parkinson's disease. In the SNpc, there was an increase in glutamate release to TH(-) dendrites and a decrease in terminals contacting TH(+) dendrites. However, in the SNpr, there was a decrease in glutamate release to both TH(+) and TH(-) dendrites.
Loss of nigrostriatal dopamine (DA) in Parkinson's disease results in over-activation/bursting of the subthalamic nucleus (STN). The STN projects to the substantia nigra (SN) pars compacta (SNpc) and pars reticulata (SNpr). The vesicular glutamate transporter 2 (Vglut2) is localized within at least STN terminals synapsing within the SN, but it is not known if there are differential changes in the Vglut2+ input to the SNpc versus SNpr following DA loss. The goal/rationale of this current study was to determine whether there were differential changes in the density/levels of glutamate immuno-gold labeling within Vglut2+ nerve terminals synapsing in the SNpc/SNpr and in the proportion of Vglut2+ terminals contacting tyrosine hydroxylase (TH) positively(+) or negatively(-) labeled dendrites following DA loss. Within the SNpc, there was a significant increase (51.3%) in the density of nerve terminal glutamate immuno-gold labeling within Vglut2+ terminals synapsing on TH(-) dendrites following MPTP versus the vehicle (VEH) group. There was a significant decrease (16%) in the percentage of Vglut2+ terminals contacting TH(+) labeled dendrites in the MPTP- versus VEH-treated group within the SNpc. Within the SNpr, there was a significant decrease in the density of glutamate immuno-gold labeling in Vglut2+ terminals contacting TH(+) (71.5%) and TH(-) (55.5%) labeled dendrites, suggesting an increase in glutamate release. There was no change in the percentage of Vglut2+ terminals contacting TH(+) or TH(-) dendrites in the SNpr. We conclude that there is a differential effect following DA loss on the glutamate input from Vglut2+ terminals synapsing within the SNpr versus SNpc.

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