Spinocerebellar Ataxia Type 1 Characteristics in Patient‐Derived Fibroblast and <scp>iPSC</scp>‐Derived Neuronal Cultures-Reference-Cited by-同舟云学术

Spinocerebellar Ataxia Type 1 Characteristics in Patient‐Derived Fibroblast and iPSC‐Derived Neuronal Cultures

Published:2023-06-06 Issue:8 Volume:38 Page:1428-1442
ISSN:0885-3185
Container-title:Movement Disorders
language:en
Short-container-title:Movement Disorders

Author:

Buijsen Ronald A.M.¹^ORCID,Hu Michel¹²^ORCID,Sáez‐González Maria¹^ORCID,Notopoulou Sofia³^ORCID,Mina Eleni¹^ORCID,Koning Winette¹^ORCID,Gardiner Sarah L.¹²,van der Graaf Linda M.¹^ORCID,Daoutsali Elena¹^ORCID,Pepers Barry A.¹^ORCID,Mei Hailiang⁴^ORCID,van Dis Vera⁵⁶,Frimat Jean‐Philippe¹²^ORCID,van den Maagdenberg Arn M. J. M.¹²^ORCID,Petrakis Spyros³^ORCID,van Roon‐Mom Willeke M.C.¹^ORCID

Affiliation:

1. Department of Human Genetics Leiden University Medical Center Leiden Zuid‐Holland The Netherlands

2. Department of Neurology Leiden University Medical Center Leiden Zuid‐Holland The Netherlands

3. Institute of Applied Biosciences, Centre for Research and Technology Hellas Thessaloniki Greece

4. Department of Biomedical Data Sciences Leiden University Medical Center Leiden Zuid‐Holland The Netherlands

5. Department of Pathology Leiden University Medical Center Leiden Zuid‐Holland The Netherlands

6. Department of Pathology Erasmus Medical Center Rotterdam Zuid‐Holland The Netherlands

Abstract

AbstractBackgroundSpinocerebellar ataxia type 1 (SCA1) is a neurodegenerative disease caused by a polyglutamine expansion in the ataxin‐1 protein resulting in neuropathology including mutant ataxin‐1 protein aggregation, aberrant neurodevelopment, and mitochondrial dysfunction.ObjectivesIdentify SCA1‐relevant phenotypes in patient‐specific fibroblasts and SCA1 induced pluripotent stem cells (iPSCs) neuronal cultures.MethodsSCA1 iPSCs were generated and differentiated into neuronal cultures. Protein aggregation and neuronal morphology were evaluated using fluorescent microscopy. Mitochondrial respiration was measured using the Seahorse Analyzer. The multi‐electrode array (MEA) was used to identify network activity. Finally, gene expression changes were studied using RNA‐seq to identify disease‐specific mechanisms.ResultsBioenergetics deficits in patient‐derived fibroblasts and SCA1 neuronal cultures showed altered oxygen consumption rate, suggesting involvement of mitochondrial dysfunction in SCA1. In SCA1 hiPSC‐derived neuronal cells, nuclear and cytoplasmic aggregates were identified similar in localization as aggregates in SCA1 postmortem brain tissue. SCA1 hiPSC‐derived neuronal cells showed reduced dendrite length and number of branching points while MEA recordings identified delayed development in network activity in SCA1 hiPSC‐derived neuronal cells. Transcriptome analysis identified 1050 differentially expressed genes in SCA1 hiPSC‐derived neuronal cells associated with synapse organization and neuron projection guidance, where a subgroup of 151 genes was highly associated with SCA1 phenotypes and linked to SCA1 relevant signaling pathways.ConclusionsPatient‐derived cells recapitulate key pathological features of SCA1 pathogenesis providing a valuable tool for the identification of novel disease‐specific processes. This model can be used for high throughput screenings to identify compounds, which may prevent or rescue neurodegeneration in this devastating disease. © 2023 The Authors. Movement Disorders published by Wiley Periodicals LLC on behalf of International Parkinson and Movement Disorder Society.

Funder

Hersenstichting

Publisher

Wiley

Subject

Neurology (clinical),Neurology

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