Background: Loss of substantia nigra dopaminergic cells and alpha-synuclein (alpha-syn)-rich intraneuronal deposits within the central nervous system are key hallmarks of Parkinson's disease (PD). Levodopa (L-DOPA) is the current gold-standard treatment for PD. This study aimed to evaluate in vivo retinal changes in a transgenic PD model of alpha-syn overexpression and the effect of acute levodopa (L-DOPA) treatment. Methods: Anaesthetised 6-month-old mice expressing human A53T alpha-synuclein (HOM) and wildtype (WT) control littermates were intraperitoneally given 20 mg/kg L-DOPA (50 mg levodopa, 2.5 mg benserazide) or vehicle saline (n = 11-18 per group). In vivo retinal function (dark-adapted full-field ERG) and structure (optical coherence tomography, OCT) were recorded before and after drug treatment for 30 min. Ex vivo immunohistochemistry (IHC) on flat-mounted retina was conducted to assess tyrosine hydroxylase (TH) positive cell counts (n = 7-8 per group). Results: We found that photoreceptor (a-wave) and bipolar cell (b-wave) ERG responses (p < 0.01) in A53T HOM mice treated with L-DOPA grew in amplitude more (47 +/- 9%) than WT mice (16 +/- 9%) treated with L-DOPA, which was similar to the vehicle group (A53T HOM 25 +/- 9%; WT 19 +/- 7%). While outer retinal thinning (outer nuclear layer, ONL, and outer plexiform layer, OPL) was confirmed in A53T HOM mice (p < 0.01), L-DOPA did not have an ameliorative effect on retinal layer thickness. These findings were observed in the absence of changes to the number of TH-positive amacrine cells across experiment groups. Acute L-DOPA treatment transiently improves visual dysfunction caused by abnormal alpha-synuclein accumulation. Conclusions: These findings deepen our understanding of dopamine and alpha-synuclein interactions in the retina and provide a high-throughput preclinical framework, primed for translation, through which novel therapeutic compounds can be objectively screened and assessed for fast-tracking PD drug discovery.
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Neurosci Res Australia, Sydney, NSW 2031, Australia
Univ New South Wales, Sydney, NSW 2031, AustraliaNeurosci Res Australia, Sydney, NSW 2031, Australia
Huang, Yue
Chegini, Fariba
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Flinders Univ S Australia, Sch Med, Dept Human Physiol, Bedford Pk, SA 5042, Australia
Flinders Univ S Australia, Sch Med, Ctr Neurosci, Bedford Pk, SA 5042, AustraliaNeurosci Res Australia, Sydney, NSW 2031, Australia
Chegini, Fariba
Chua, Germaine
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Neurosci Res Australia, Sydney, NSW 2031, Australia
Univ New South Wales, Sydney, NSW 2031, AustraliaNeurosci Res Australia, Sydney, NSW 2031, Australia
Chua, Germaine
Murphy, Karen
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Neurosci Res Australia, Sydney, NSW 2031, Australia
Univ New South Wales, Sydney, NSW 2031, AustraliaNeurosci Res Australia, Sydney, NSW 2031, Australia
Murphy, Karen
Gai, Weiping
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Flinders Univ S Australia, Sch Med, Dept Human Physiol, Bedford Pk, SA 5042, Australia
Flinders Univ S Australia, Sch Med, Ctr Neurosci, Bedford Pk, SA 5042, AustraliaNeurosci Res Australia, Sydney, NSW 2031, Australia
Gai, Weiping
Halliday, Glenda M.
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Neurosci Res Australia, Sydney, NSW 2031, Australia
Univ New South Wales, Sydney, NSW 2031, AustraliaNeurosci Res Australia, Sydney, NSW 2031, Australia
机构:
Univ Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, FinlandUniv Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, Finland
Kilpelainen, Tommi
Julku, Ulrika H.
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Univ Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, FinlandUniv Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, Finland
Julku, Ulrika H.
Svarcbahs, Reinis
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Univ Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, FinlandUniv Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, Finland
Svarcbahs, Reinis
Myohanen, Timo T.
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Univ Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, FinlandUniv Helsinki, Div Pharmacol & Pharmacotherapy, Fac Pharm, Drug Res Program, Helsinki, Finland