4.6 Article

Tumorigenicity analysis of heterogeneous dental stem cells and its self-modification for chromosome instability

Journal

CELL CYCLE
Volume 14, Issue 21, Pages 3396-3407

Publisher

TAYLOR & FRANCIS INC
DOI: 10.1080/15384101.2015.1036204

Keywords

aneuploidy; cell-based therapy; CIN; DFSCs; heterogeneity

Categories

Funding

  1. National Basic Research Program (China) [2010CB944800]
  2. Nature Science Foundation (China) [81271095, 81271119, 81200792, 81300848]
  3. International Cooperation Program of China (China) [2013DFG32770, 2011DFA51970]
  4. Trans-Century Training Pro-gramme Foundation for the Talents of Humanities and Social Science by the State Eduation Commission (China) [NCET-13-0385]
  5. Doctoral Foundation of Ministry of Education (China) [20110181120067, 20110181110089, 20120181120013]
  6. China postdoctoral science foundation (China) [2012M511934]
  7. Key Technology R&D Program of Sichuan Province [2010FZ0055, 2012SZ0013, 12ZC0493, 13ZC0971, 2013GZX0158, 2013SZ0015, 13ZC0979]
  8. Basic Research Program of Sichuan Province [2011JY0125, 12JC0212, 2012JY0077, 2013JY0019]

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Heterogeneity demonstrates that stem cells are constituted by several sub-clones in various differentiation states. The heterogeneous state is maintained by cross-talk among sub-clones, thereby ensuring stem cell adaption. In this study, we investigated the roles of heterogeneity on genetic stability. Three sub-clones (DF2, DF8 and DF18) were isolated from heterogeneous dental stem cells (DSCs), and were proved to be chromosome instability (CIN) after long term expansion. Cell apoptosis were not detected in sub-clones, which exhibited strong tumorigenesis tendency, coupled with weak expression of p53 and aberrant ultra-structure. However, 3 sub-clones did not overexpress tumor related markers or induce tumorigenesis in vivo. The mixed-culture study suggested that 3-clone-mixed culturing cells (DF1) presented apparent decrease in the ratio of aneuploidy. The screening experiment further proved that 3 sub-clones functioned separately in this modification procedure but only mixed culturing all 3 sub-clones, simulated heterogeneous microenvironment, could achieve complete modification. Additionally, osteogenesis capability of 3 sub-clones was partially influenced by CIN while DSCs still kept stronger osteogenesis than sub-clones. These results suggested aberrant sub-clones isolated from heterogeneous DSCs were not tumorigenesis and could modify CIN by cross-talk among themselves, indicating that the heterogeneity played a key role in maintaining genetic stability and differentiation capability in dental stem cells.

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