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Selection of iPSCs without mtDNA deletion for autologous cell therapy in a patient with Pearson syndrome

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Abstract
Screening for genetic defects in the cells should be examined for clinical application. The Pearson syndrome (PS) patient harbored nuclear mutations in the POLG and SSBP1 genes, which could induce systemic large-scale mitochondrial genome (mtDNA) deletion. We investigated iPSCs with mtDNA deletions in PS patient and whether deletion levels could be maintained during differentiation. The iPSC clones derived from skin fibroblasts (9% deletion) and blood mononuclear cells (24% deletion) were measured for mtDNA deletion levels. Of the 13 skin-derived iPSC clones, only 3 were found to be free of mtDNA deletions, whereas all blood-derived iPSC clones were found to be free of deletions. The iPSC clones with (27%) and without mtDNA deletion (0%) were selected and performed in vitro and in vivo differentiation, such as embryonic body (EB) and teratoma formation. After differentiation, the level of deletion was retained or increased in EBs (24%) or teratoma (45%) from deletion iPSC clone, while, the absence of deletions showed in all EBs and teratomas from deletion-free iPSC clones. These results demonstrated that non-deletion in iPSCs was maintained during in vitro and in vivo differentiation, even in the presence of nuclear mutations, suggesting that deletion-free iPSC clones could be candidates for autologous cell therapy in patients.
Author(s)
Selection of iPSCs without mtDNA deletion for autologous cell therapy in a patient with Pearson syndrome
Issued Date
2023
Yeonmi Lee
Jongsuk Han
Sae-Byeok Hwang
Soon-Suk Kang
Hyeoung-Bin Son
Chaeyeon Jin
Jae Eun Kim
Beom Hee Lee
Eunju Kang
Type
Article
Keyword
EB formationiPSCsmtDNA deletionPS patientTeratoma formation
DOI
10.5483/BMBRep.2022-0204
URI
https://oak.ulsan.ac.kr/handle/2021.oak/17060
Publisher
BMB Reports
Language
영어
ISSN
1976-6696
Citation Volume
56
Citation Number
8
Citation Start Page
463
Citation End Page
468
Appears in Collections:
Medicine > Nursing
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