Acyclic retinoid induces differentiation and apoptosis of murine hepatic stem cells

The therapeutic potential of acyclic retinoid (ACR), a synthetic retinoid, has been confirmed in experimental and clinical studies. Therapeutic targets include precancerous and cancer stem cells. As ACR is also involved in developmental processes, its effect on normal hepatic stem cells (HpSCs) shou...

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Published in:Stem cell research & therapy 2015-03, Vol.6 (1), p.51-51, Article 51
Main Authors: Guan, Hong-Bin, Nie, Yun-Zhong, Zheng, Yun-Wen, Takiguchi, Kazuya, Yu, Hong-Wei, Zhang, Ran-Ran, Li, Bin, Tsuchida, Tomonori, Taniguchi, Hideki
Format: Article
Language:English
Subjects:
alpha-Fetoproteins - biosynthesis
Analysis
Animals
Annexin A5 - biosynthesis
Apoptosis
Apoptosis - drug effects
Cancer
Caspase 3 - biosynthesis
Cell differentiation
Cell Differentiation - drug effects
Cells, Cultured
Down-Regulation
Flow Cytometry
Gene expression
Gene Products, tat - biosynthesis
Genes
Health aspects
Hyaluronan Receptors - biosynthesis
Intercellular Signaling Peptides and Proteins - biosynthesis
Liver - cytology
Liver Regeneration - physiology
Medical colleges
Mice
Mice, Inbred C57BL
Oncology, Experimental
Physiological aspects
Receptors, Retinoic Acid - metabolism
Stem cells
Stem Cells - cytology
Stem Cells - metabolism
Tretinoin - analogs & derivatives
Tretinoin - pharmacology
Up-Regulation
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Summary:The therapeutic potential of acyclic retinoid (ACR), a synthetic retinoid, has been confirmed in experimental and clinical studies. Therapeutic targets include precancerous and cancer stem cells. As ACR is also involved in developmental processes, its effect on normal hepatic stem cells (HpSCs) should be investigated for understanding the underlying mechanisms. Here, we examined effects of the acyclic retinoid peretinoin on fresh isolated murine HpSCs. We isolated c-kit-CD29+CD49f+/lowCD45-Ter119- cells from murine fetal livers using flow cytometry. To evaluate the effect of ACR, we traced clonal expansion and analyzed cell differentiation as well as apoptosis during the induction process by immunofluorescent staining and marker gene expression. ACR dose-dependently inhibited HpSCs expansion. Stem cell clonal expansion was markedly inhibited during the culture period. Moreover, ACR showed a significant promotion of HpSC differentiation and induction of cellular apoptosis. The expression of stem cell marker genes, Afp, Cd44, and Dlk, was downregulated, while that of mature hepatocyte genes, Alb and Tat, and apoptosis-related genes, Annexin V and Caspase-3, were upregulated. Flow cytometry showed that the proportion of Annexin V-positive cells increased after ACR incubation compared with the control. Data obtained by immunofluorescent staining for albumin and Caspase-3 corroborated the data on gene expression. Finally, we found that ACR directly regulates the expression of retinoic acid receptors and retinoid X receptors. These findings indicate that ACR inhibits the clonal expansion of normal HpSCs in vitro and promotes the differentiation of immature cells by regulating receptors of retinoic acid.
ISSN:1757-6512
1757-6512
DOI:10.1186/s13287-015-0046-9