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Maintenance of hPSCs under Xeno-Free and Chemically Defined Culture Conditions

Authors
Lim, Jung JinKim, Hyung JoonRhie, Byung-hoLee, Man RyulChoi, Myeong JunHong, Seok-HoKim, Kye-Seong
Issue Date
Nov-2019
Publisher
Korean Society for Stem Cell Research
Keywords
Embryonic stem cells; Induced pluripotent stem cells; Feeder-free; Chemically defined conditions; Extracellular matrices
Citation
International Journal of Stem Cells, v.12, no.3, pp 484 - 496
Pages
13
Journal Title
International Journal of Stem Cells
Volume
12
Number
3
Start Page
484
End Page
496
URI
https://scholarworks.bwise.kr/sch/handle/2021.sw.sch/4105
DOI
10.15283/ijsc19090
ISSN
2005-3606
2005-5447
Abstract
Previously, the majority of human embryonic stem cells and human induced pluripotent stem cells have been derived on feeder layers and chemically undefined medium. Those media components related to feeder cells, or animal products, often greatly affect the consistency of the cell culture. There are clear advantages of a defined, xeno-free, and feeder-free culture system for human pluripotent stem cells (hPSCs) cultures, since consistency in the formulations prevents lot-to-lot variability. Eliminating all non-human components reduces health risks for downstream applications, and those environments reduce potential immunological reactions from stem cells. Therefore, development of feeder-free hPSCs culture systems has been an important focus of hPSCs research. Recently, researchers have established a variety of culture systems in a defined combination, xeno-free matrix and medium that supports the growth and differentiation of hPSCs. Here we described detailed hPSCs culture methods under feeder-free and chemically defined conditions using vitronetin and TeSR-E8 medium including supplement bioactive lysophospholipid for promoting hPSCs proliferation and maintaining stemness.
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