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Efficient gene delivery in differentiated human embryonic stem cells
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  • Published: 01 February 2005

Efficient gene delivery in differentiated human embryonic stem cells

  • Jae-Hwan Kim1,
  • Hyun-Jin Do,
  • Seong-Jun Choi,
  • Hyun-Jung Cho,
  • Kyu-Hyung Park,
  • Heung-Mo Yang,
  • Sang-Hwa Lee,
  • Dong-Ku Kim,
  • KyuBum Kwack,
  • Sun-Kyung Oh,
  • Shin-Yong Moon,
  • Kwang-Yul Cha &
  • …
  • Hyung-Min Chung 

Experimental & Molecular Medicine volume 37, pages 36–44 (2005)Cite this article

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  • 26 Citations

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An Erratum to this article was published on 01 October 2006

Abstract

Human embryonic stem (hES) cells are capable of differentiating into pluralistic cell types, however, spontaneous differentiation generally gives rise to a limited number of specific differentiated cell types and a large degree of cell heterogeneity. In an effort to increase the efficiency of specified hES cell differentiation, we performed a series of transient transfection of hES cells with EGFP expression vectors driven by different promoter systems, including human cellular polypeptide chain elongation factor 1 α (hEF1α), human cytomegalo-virus, and chicken β-actin. All these promoters were found to lead reporter gene expression in undifferentiated hES cells, but very few drug-selectable transfectants were obtained and failed to maintain stable expression of the transgene with either chemical or electroporation methods. In an attempt to increase transfection efficiency and obtain stable transgene expression, differentiated hES cells expressing both mesodermal and ectodermal markers were derived using a defined medium. Differentiated hES cells were electroporated with a hEF1α promoter-driven EGFP or human noggin expression vector. Using RT-PCR, immunocytochemistry and fluorescence microscopy, the differentiated hES cells transfected with foreign genes were confirmed to retain stable gene and protein expression during prolonged culture. These results may provide a new tool for introducing exogenous genes readily into hES cells, thereby facilitating more directed differentiation into specific and homogenous cell populations.

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Authors and Affiliations

  1. Cell and Gene Therapy Research Institute, Pochon CHA University, Gangweondo, Korea

    Jae-Hwan Kim

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  1. Jae-Hwan Kim
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  2. Hyun-Jin Do
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  3. Seong-Jun Choi
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  4. Hyun-Jung Cho
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  5. Kyu-Hyung Park
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  6. Heung-Mo Yang
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  7. Sang-Hwa Lee
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  8. Dong-Ku Kim
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  9. KyuBum Kwack
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  10. Sun-Kyung Oh
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  11. Shin-Yong Moon
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  12. Kwang-Yul Cha
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  13. Hyung-Min Chung
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This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

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Cite this article

Kim, JH., Do, HJ., Choi, SJ. et al. Efficient gene delivery in differentiated human embryonic stem cells. Exp Mol Med 37, 36–44 (2005). https://doi.org/10.1038/emm.2005.5

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  • Published: 01 February 2005

  • Issue date: 01 February 2005

  • DOI: https://doi.org/10.1038/emm.2005.5

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Keywords

  • differentiation
  • embryoid body
  • human embryonic stem cell
  • promoter
  • RT-PCR
  • transfection

This article is cited by

  • Comparison of Gene-Transfer Efficiency in Human Embryonic Stem Cells

    • Feng Cao
    • Xiaoyan Xie
    • Joseph C. Wu

    Molecular Imaging and Biology (2010)

  • Human Embryonic Stem Cells and Gene Therapy

    • Yael Strulovici
    • Philip L Leopold
    • Ronald G Crystal

    Molecular Therapy (2007)

  • Progress and prospects: gene transfer into embryonic stem cells

    • F Yates
    • G Q Daley

    Gene Therapy (2006)

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Experimental & Molecular Medicine (Exp Mol Med)

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ISSN 1226-3613 (print)

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