Iranian South Medical Journal (Oct 2014)

Generation of hematopoietic lineage cells from embryonic like cells

  • Gholam Reza Khamisipour,
  • Ali Akbar Pourfathollah,
  • Masoud Soleimani,
  • Mehdi Fourouzandeh Moghaddam,
  • Mehrdad Norouzinia,
  • Said Kavyani,
  • Kamran Ali Moghaddam,
  • Gholam Reza Heydari,
  • Hamid Reza Alizadeh-Otaghvar

Journal volume & issue
Vol. 17, no. 4
pp. 506 – 516

Abstract

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Background: Epigenetic reprogramming of somatic cells into embryonic stem cells has attracted much attention, because of the potential for stem cell transplantation and compatibility with recipient. However, the therapeutic application of either nuclear transfer or nuclear fusion of somatic cell has been hindered by technical complications as well as ethical objections. Recently, a new method is reported whereby ectopic expression of embryonic specific transcription factors was shown to induce fibroblasts to become embryonic like SCs (induced pluripotent stem cells). A major limitation of this method is the use of potentially harmful genome integrating viruses such as reto- or lentivirus. The main aim of this investigation was generation of human hematopoietic stem cells from induced fibroblasts by safe adenovectors carrying embryonically active genes. Material and Methods: Isolated fibroblasts from foreskin were expanded and recombinant adenoviruses carrying human Sox2, Oct4, Klf4, cMyc genes were added to culture. After formation of embryonic like colonies and cell expansion, they were transferred to embryonic media without bFGF, and embryoid bodies were cultured on stromal and non-stromal differentiation media for 14 days. Results: Expression of CD34 gene and antigenic markers, CD34, CD38 & CD133 in stromal culture showed significant difference with non-differentiation and non-stromal media. Conclusion: These findings show high hematopoietic differentiation rate of Adeno-iPS cells in stromal culture and no need to use growth factors. While, there was no difference between non-differentiation and non-stromal media.

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