Generation of hematopoietic stem cells from human embryonic stem cells using a defined, stepwise, serum-free, and serum replacement-free monolayer culture method.

So Jung Kim; Ji Won Jung; Hye Yeong HA; Soo Kyung Koo; Eung Gook Kim; Jung Hyun Kim

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Generation of hematopoietic stem cells from human embryonic stem cells using a defined, stepwise, serum-free, and serum replacement-free monolayer culture method.

Author: So Jung KIM ¹ ; Ji Won JUNG ; Hye Yeong HA ; Soo Kyung KOO ; Eung Gook KIM ; Jung Hyun KIM
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1. Division of Intractable Diseases, Center for Biomedical Sciences, National Institute of Health and Korea Centers for Diseases Control and Prevention, Cheongju, Korea. kjhcorea@korea.kr
Publication Type:Original Article
Keywords: Pluripotent stem cell; Hematopoietic differentiation; Xeno-free protocol
MeSH: Animals; Cytokines; Embryonic Stem Cells; Hematopoietic Stem Cells*; Human Embryonic Stem Cells*; Humans*; In Vitro Techniques; Methods*; Pluripotent Stem Cells; Stem Cells
From:Blood Research 2017;52(1):37-43
CountryRepublic of Korea
Language:English
Abstract: BACKGROUND: Embryonic stem cells (ESCs) can be expanded infinitely in vitro and have the potential to differentiate into hematopoietic stem cells (HSCs); thus, they are considered a useful source of cells for HSC production. Although several technical in vitro methods for engineering HSCs from pluripotent stem cells have been developed, clinical application of HSCs engineered from pluripotent stem cells is restricted because of the possibility of xenogeneic contamination resulting from the use of murine materials. METHODS: Human ESCs (CHA-hES15) were cultured on growth factor-reduced Matrigel-coated dishes in the mTeSR1 serum-free medium. When the cells were 70% confluent, we initiated HSC differentiation by three methods involving (1) knockout serum replacement (KSR), cytokines, TGFb1, EPO, and FLT3L; (2) KSR, cytokines, and bFGF; or (3) cytokines and bFGF. RESULTS: Among the three differentiation methods, the minimal number of cytokines without KSR resulted in the greatest production of HSCs. The optimized method resulted in a higher proportion of CD34⁺CD43⁺ hematopoietic progenitor cells (HPCs) and CD34⁺CD45⁺ HPCs compared to the other methods. In addition, the HSCs showed the potential to differentiate into multiple lineages of hematopoietic cells in vitro. CONCLUSION: In this study, we optimized a two-step, serum-free, animal protein-free, KSR-free, feeder-free, chemically defined monolayer culture method for generation of HSCs and hematopoietic stem and progenitor cells (HSPCs) from human ESCs.