4.6 Article

A Practical and Efficient Cellular Substrate for the Generation of Induced Pluripotent Stem Cells from Adults: Blood-Derived Endothelial Progenitor Cells

STEM CELLS TRANSLATIONAL MEDICINE (2012)

Get Full Text
Add to Collection

Journal

STEM CELLS TRANSLATIONAL MEDICINE
Volume 1, Issue 12, Pages 855-865

Publisher

ALPHAMED PRESS
DOI: 10.5966/sctm.2012-0093

Keywords

Induced pluripotent stem cells; Endothelial cell; Progenitor cells; Reprogramming; Direct cell conversion

Categories

Cell & Tissue Engineering

Funding

  1. British Heart Foundation [RG/08/002/24718]
  2. Medical Research Council [G1000847, 85198]
  3. Wellcome Trust [098051, 090660/Z/09/Z]
  4. Fondation Leducq
  5. Cambridge Cardiovascular Consortium
  6. Cambridge NIHR Biomedical Research Centre
  7. Cambridge Stem Cell Institute
  8. Pfizer
  9. Academy of Medical Sciences (AMS) [AMS-SGCL5-Toshner] Funding Source: researchfish
  10. British Heart Foundation [FS/12/39/29653, RG/08/002/24718] Funding Source: researchfish
  11. Medical Research Council [G0800784, G1000847] Funding Source: researchfish
  12. National Institute for Health Research [NF-SI-0509-10174] Funding Source: researchfish
  13. Wellcome Trust [090660/Z/09/Z] Funding Source: Wellcome Trust
  14. MRC [G0800784, G1000847] Funding Source: UKRI

Ask authors/readers for more resources

Protocol

Community support

Reagent

Community support

Induced pluripotent stem cells (iPSCs) have the potential to generate patient-specific tissues for disease modeling and regenerative medicine applications. However, before iPSC technology can progress to the translational phase, several obstacles must be overcome. These include uncertainty regarding the ideal somatic cell type for reprogramming, the low kinetics and efficiency of reprogramming, and karyotype discrepancies between iPSCs and their somatic precursors. Here we describe the use of late-outgrowth endothelial progenitor cells (L-EPCs), which possess several favorable characteristics, as a cellular substrate for the generation of iPSCs. We have developed a protocol that allows the reliable isolation of L-EPCs from peripheral blood mononuclear cell preparations, including frozen samples. As a proof-of-principle for clinical applications we generated EPC-iPSCs from both healthy individuals and patients with heritable and idiopathic forms of pulmonary arterial hypertension. L-EPCs grew clonally; were highly proliferative, passageable, and bankable; and displayed higher reprogramming kinetics and efficiencies compared with dermal fibroblasts. Unlike fibroblasts, the high efficiency of L-EPC reprogramming allowed for the reliable generation of iPSCs in a 96-well format, which is compatible with high-throughput platforms. Array comparative genome hybridization analysis of L-EPCs versus donor-matched circulating monocytes demonstrated that L-EPCs have normal karyotypes compared with their subject's reference genome. In addition, >80% of EPC-iPSC lines tested did not acquire any copy number variations during reprogramming compared with their parent L-EPC line. This work identifies L-EPCs as a practical and efficient cellular substrate for iPSC generation, with the potential to address many of the factors currently limiting the translation of this technology. STEM CELLS TRANSLATIONAL MEDICINE 2012;1:855-865

Authors

I am an author on this paper
Click your name to claim this paper and add it to your profile.

Reviews

Primary Rating

4.6
Not enough ratings

Secondary Ratings

Novelty
-
Significance
-
Scientific rigor
-
Rate this paper

Recommended

No Data Available
No Data Available
Webinars Posters Questions Hubs Funding Journals Papers Connect Collections Reviewers About Us FAQs Mobile App Privacy Policy Terms of Use
© Peeref 2019-2024. All rights reserved.