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Transcriptomic insights and feeder-free culturing of porcine expanded potential stem cells from cloned embryosopen access

Authors
Cai, LianKim, MiraeChoi, HyerinKim, HaneulHyun, Sang-HwanKim, Eunhye
Issue Date
Sep-2025
Publisher
BioMed Central
Keywords
Expanded pluripotent stem cell; Porcine embryos; Somatic cell nuclear transfer; Feeder-free culture
Citation
Stem Cell Research & Therapy, v.16, no.1
Indexed
SCIE
SCOPUS
Journal Title
Stem Cell Research & Therapy
Volume
16
Number
1
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/80957
DOI
10.1186/s13287-025-04627-5
ISSN
1757-6512
1757-6512
Abstract
Background Generating expanded potential stem cells from cloned porcine embryos (pEPSCsNT) represents a notable advancement in regenerative medicine and agricultural biotechnology. However, challenges, including low derivation efficiency, limited understanding of transcriptomic features, and unknown feasibility of culturing under feeder-free conditions, remain. This study aimed to generate pEPSCs using blastocysts derived from parthenogenetic activation, in vitro fertilization, and somatic cell nuclear transfer (SCNT) using a modified culture system. Methods We derived pEPSCNT lines using an optimized culture system. We characterized the pEPSC lines from all three origins by analyzing pluripotent marker expression, performing karyotyping, and assessing their differentiation potential into the three germ layers. Furthermore, we performed a comparative transcriptomic analysis using in vivo and cloned embryo data, with a major focus on cell lines derived from SCNT (pEPSCsNT). We optimized feeder-free culture conditions for the pEPSCNT line and derived the pEPSCNT lines using an optimized culture system with an efficiency of similar to 14%. Results The cells were closely correlated with 8-cell to morula-stage embryos and exhibited significant enrichment of EPSC signature genes, suggesting a unique pluripotent state relatively close to the naive state, specifically within a formative state. The pEPSCsNT possessed broad differentiation capacity, indicative of Hippo signaling pathway enrichment, blastocyst-like structure formation ability, and potential differentiation into trophoblast lineage cells. Conclusions Our modified culture medium combined with the 2x Matrigel coating system facilitated the transition to feeder-independent culture conditions. These findings facilitate the establishment of a feeder-free culture system while preserving pluripotency and differentiation potential.
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