Identification and selection of cardiomyocytes during human embryonic stem cell differentiation

被引:191
作者
Huber, Irit
Itzhaki, Ilanit
Caspi, Oren
Arbel, Gil
Tzukerman, Maty
Gepstein, Amira
Habib, Manhal
Yankelson, Lior
Kehat, Izhak
Gepstein, Lior
机构
[1] Technion Israel Inst Technol, Bruce Rappaport Fac Med, Sohis Family Res Lab Regenerat Funct Myocardium, IL-31096 Haifa, Israel
[2] Technion Israel Inst Technol, Bruce Rappaport Fac Med, Rappaport Family Inst Res Med Sci, IL-31096 Haifa, Israel
关键词
myogenesis; myosin light chain 2-V; promoter; selectable marker; embryoid body; cardiac differentiation;
D O I
10.1096/fj.05-5711com
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Human embryonic stem cells (hESC) are pluripotent lines that can differentiate in vitro into cell derivatives of all three germ layers, including cardiomyocytes. Successful application of these unique cells in the areas of cardiovascular research and regenerative medicine has been hampered by difficulties in identifying and selecting specific cardiac progenitor cells from the mixed population of differentiating cells. We report the generation of stable transgenic hESC lines, using lentiviral vectors, and single-cell clones that express a reporter gene (eGFP) under the transcriptional control of a cardiac-specific promoter (the human myosin light chain-2V promoter). Our results demonstrate the appearance of eGFP-expressing cells during the differentiation of the hESC as embryoid bodies (EBs) that can be identified and sorted using FACS (purity > 95%, viability > 85%). The eGFP-expressing cells were stained positively for cardiac-specific proteins (> 93%), expressed cardiac-specific genes, displayed cardiac-specific action-potentials,and could form stable myocardial cell grafts following in vivo cell transplantation. The generation of these transgenic hESC lines may be used to identify and study early cardiac precursors for developmental studies, to robustly quantify the extent of cardiomyocyte differentiation, to label the cells for in vivo grafting, and to allow derivation of purified cell populations of cardiomyocytes for future myocardial cell therapy strategies.
引用
收藏
页码:2551 / 2563
页数:13
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