Abstract
Human induced pluripotent stem (hiPS) cells provide therapeutic promises, as well as a potent in vitro model for studying biological processes that take place during human embryonic development and subsequent differentiation in normal and disease states. The epigenetic characteristics of iPS cells are reprogrammed to the embryonic state at which they acquire pluripotency. In addition, telomeres in hiPS cell must elongate sufficiently to provide the necessary replicative potential. Recent studies have demonstrated that the epigenetic characteristics of telomeric and subtelomeric regions are pivotal in regulating telomere length. Here we study telomere length, subtelomeric DNA methylation and telomeric-repeat-containing RNA (TERRA) expression in several hiPS cell clones derived from normal neonatal foreskin fibroblasts. We find that telomeres lengthen significantly in hiPS cells in comparison to the parental fibroblast source, and progressively shorten after differentiation back into fibroblast-like cells, concomitantly with telomerase activation and downregulation, respectively. Subtelomeres in hiPS cells were found to be generally hypermethylated in comparison to the parental source. However, bisulfite analysis revealed that at several subtelomeres examined, methylation levels differed between hiPS clones and that both de novo methylation and demethylation processes occurred during telomere reprogramming. Notably, although subtelomeres were in general very highly methylated, TERRA levels were elevated in hiPS cells, albeit to different degrees in the various clones. TERRA elevation may reflect enhanced stability or impaired degradation in hiPS cells, and/or alternatively, increased transcription from the hypomethylated subtelomeres. We suggest that TERRA may play a role in regulation of appropriate telomere function and length in hiPS cells.
| Original language | English |
|---|---|
| Pages (from-to) | 63-75 |
| Number of pages | 13 |
| Journal | Epigenetics |
| Volume | 6 |
| Issue number | 1 |
| DOIs | |
| State | Published - Jan 2011 |
| Externally published | Yes |
Bibliographical note
Funding Information:We are grateful to Gil Arbel, Amira Gepstein and Yeela Shamai for help in tissue culturing, to Michal Levy for help with bisulfite sequence analysis, to Liron Berger for help with confocal microscopy, to Rita Fuhrer-Mor for her excellent service in DNA sequencing and to Noa Gil for her help in bisulfite analysis. We thank Daniel Kornitzer for comments on the manuscript. This research was supported in part by The Legacy Heritage Bio-Medical Program of the Israel Science Foundation (grant No. 725/09-S.S. and grant No. 1225/09-L.G.), Arthur and Rosalinde Gilbert Foundation of the American Technion Society and Richard D. Satell Fund of the American Technion Society (K.S.).
Funding
We are grateful to Gil Arbel, Amira Gepstein and Yeela Shamai for help in tissue culturing, to Michal Levy for help with bisulfite sequence analysis, to Liron Berger for help with confocal microscopy, to Rita Fuhrer-Mor for her excellent service in DNA sequencing and to Noa Gil for her help in bisulfite analysis. We thank Daniel Kornitzer for comments on the manuscript. This research was supported in part by The Legacy Heritage Bio-Medical Program of the Israel Science Foundation (grant No. 725/09-S.S. and grant No. 1225/09-L.G.), Arthur and Rosalinde Gilbert Foundation of the American Technion Society and Richard D. Satell Fund of the American Technion Society (K.S.).
| Funders | Funder number |
|---|---|
| American Technion Society | |
| Israel Science Foundation | 725/09-S, 1225/09-L |
Keywords
- DNA methylation
- Human induced pluripotent stem cells
- Subtelomeres
- TERRA
- Telomerase
- Telomeres
