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Activin-A 처리에 의해 분화 촉진된 인간 배아 줄기세포 유래 내배엽성 세포의 효과적인 정제

Effective Isolation of Endodermal Lineage Cells Derived from Human embryonic Stem Cells Post Activin-A Treatment

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  • URLhttps://db.koreascholar.com/Article/Detail/163404
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한국동물번식학회 (The Korean Society of Animal Reproduction)
초록

Embryoid bodies (EBs) generated from human embryonic stem cells (hESCs) include spontaneously induced endodermal lineage cells (ELCs). Activin-A plays important roles in the endoderm differentiation of hESCs. Despite studies on the generation of ELCs from hESCs with treatment of Actvin-A, it was unclear for localization and pattern of ELCs by Activin-A during differentiation of hESCs. Accordingly in this study, we knew that Actvin-A increased the cystic EBs formation, including the highly enriched AFP (endoderm lineage specific marker)-expressing cells in the surface of cystic EBs. To induce the EBs formation from undifferentiated hESCs, cells were transferred onto petri-dish and cultured in suspension condition without bFGF removed hESC media (EB media) for 3 days. Next to investigate the effect of Activin-A, EBs were subsequently cultured in EB media supplement with 100 ng/ml Activin-A for 3 days. After 5~7 days of Activin-A treatment, cystic EBs began to appear which increased in numbers reaching ~60% of initially formed EBs over 5 days. Endoderm lineage marker, AFP were highly expressed and specifically localized at the surface region of cystic EBs comparison with normal EBs. We next attached the cystic EBs onto gelatin-coated plates and cultured for 5 days. In the results of real-time PCR and immunocytochemistry analysis, AFP-expressing cells migrated and localized at the outgrowth region of attached cystic EBs. To obtain the AFP-expressing cells of the outgrowth region, we manually isolated by using micro- dissection and cultured them. These cells strongly express AFP over 70% of isolated cells post re-plating. Here, we first showed an expression pattern of specifically localized ELCs by Activin-A during differentiation of hESCs. From this observation, we could highly purified ELCs from undifferentiated hESCs. Taken together, our system will provide a novel and efficient option to generate ELCs from hESCs.

목차
ABSTRACT   서론   재료 및 방법    배상체 형성 및 내배엽성 세포로의 분화    내배엽성 세포의 정제 및 배양    RNA 추출 및 실시간 중합효소 연쇄 반응 분석    면역 염색 분석    통계처리 및 분석   결과    Actvin-A가 배상체 형성에 미치는 형태학적 분석    Activin-A에 의한 배상체 내에서의 내배엽성 세포의 발현 패턴 및 분포도 분석    부착된 배상체에서의 AFP발현 패턴을 이용한 고순도 내배엽성 세포의 정제   고찰   인용문헌
저자
  • 김문규(치외과대학 의생명과학대학원 줄기세포 연구실) | Mun-Kyu Kim
  • 문성환(차바이오앤디오스텍) | Sung-Hwan Moon
  • 박순경(치외과대학 의생명과학대학원 줄기세포 연구실) | Toon-Jung Park
  • 이경일(차바이오앤디오스텍) | Kyung-Il Lee
  • 신정민(차바이오앤디오스텍) | Jeong-Min Shin
  • 장재우(치외과대학 의생명과학대학원 줄기세포 연구실) | Jae-Woo Jang
  • 정형민(치외과대학 의생명과학대학원 줄기세포 연구실, 차바이오앤디오스텍) | Hyung-Min Chung Corresponding author