Transdifferentiation of mesenchymal stem cells-derived adipogenic-differentiated cells into osteogenic- or chondrogenic-differentiated cells proceeds via dedifferentiation and have a correlation with cell cycle arresting and driving genes

Mujib Ullah; Stefan Stich; Michael Notter; Jan Eucker; Michael Sittinger; Jochen Ringe

doi:10.1016/j.diff.2013.02.001

Transdifferentiation of mesenchymal stem cells-derived adipogenic-differentiated cells into osteogenic- or chondrogenic-differentiated cells proceeds via dedifferentiation and have a correlation with cell cycle arresting and driving genes

Differentiation. 2013 Feb;85(3):78-90. doi: 10.1016/j.diff.2013.02.001. Epub 2013 May 3.

Authors

Mujib Ullah¹, Stefan Stich, Michael Notter, Jan Eucker, Michael Sittinger, Jochen Ringe

Affiliation

¹ Tissue Engineering Laboratory & Berlin-Brandenburg Center for Regenerative Therapies, Dept. of Rheumatology and Clinical Immunology, Charité-University Medicine Berlin, Charitéplatz 1, 10117 Berlin, Germany. mujib.ullah@charite.de

PMID: 23644554
DOI: 10.1016/j.diff.2013.02.001

Abstract

It is generally accepted that after differentiation bone marrow mesenchymal stem cells (MSC) become lineage restricted and unipotent in an irreversible manner. However, current results imply that even terminally differentiated cells transdifferentiate across lineage boundaries and therefore act as a progenitor cells for other lineages. This leads to the questions that whether transdifferentiation occurs via direct cell-to-cell conversion or dedifferentiation to a progenitor cells and subsequent differentiation, and whether MSC potency decreases or increases during differentiation. To address these questions, MSC were differentiated into adipogenic lineage cells, followed by dedifferentiation. The process of dedifferentiation was also confirmed by single cell clonal analysis. Finally the dedifferentiated cells were used for adipogenesis, osteogenesis and chondrogenesis. Histology, FACS, qPCR and GeneChip analyses of undifferentiated MSC, adipogenic-differentiated and dedifferentiated cells were performed. Interestingly, gene profiling and bioinformatics demonstrated that upregulation (DHCR24, G0S2, MAP2K6, SESN3) and downregulation (DST, KAT2, MLL5, RB1, SMAD3, ZAK) of distinct genes have an association with cell cycle arrest in adipogenic-differentiated cells and perhaps narrow down the lineage potency. However, the upregulation (CCND1, CHEK, HGF, HMGA2, SMAD3) and downregulation (CCPG1, RASSF4, RGS2) of these genes have an association with cell cycle progression and maybe motivate dedifferentiation of adipogenic-differentiated cells. We found that dedifferentiated cells have a multilineage potency comparable to MSC, and also observed the associative role of proliferation genes with cell cycle arrest and progression. Concluded, our results indicate that transdifferentiation of adipogenic-differentiated cells into osteogenic- or chondrogenic-differentiated cells proceeds via dedifferentiation and correlates with cell cycle arresting and deriving genes. Regarding clinical use, the knowledge of potency and underlying mechanisms are prerequisites.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adipose Tissue / cytology*
Bone Marrow Cells / cytology
Cell Cycle Checkpoints / genetics
Cell Dedifferentiation*
Cell Differentiation*
Cell Transdifferentiation*
Cells, Cultured
Chondrogenesis / genetics
Gene Expression Regulation, Developmental
Humans
Mesenchymal Stem Cells / cytology*
Oligonucleotide Array Sequence Analysis
Osteogenesis / genetics
Stem Cells / cytology
Up-Regulation