利用甲胎蛋白启动子活力筛选人胚胎肝脏前体细胞

doi:10.3969/j.issn.0529-1356.2011.01.008

›› 2011, Vol. 42 ›› Issue (1): 45-49.doi: 10.3969/j.issn.0529-1356.2011.01.008

利用甲胎蛋白启动子活力筛选人胚胎肝脏前体细胞

王萍^{1, 2; 刘保清^{1 ;李卫红^{1 ;董凌月^{1 ;尤红^{2 ;贾继东^{2 ;安威^{1 ;张海燕^1*}}}}}}}

1.首都医科大学细胞生物学系，北京市肝脏保护与再生调节重点实验室，北京 100069;2.首都医科大学附属北京友谊医院肝病研究中心，北京 100050

收稿日期:2010-01-29 修回日期:2010-06-02 出版日期:2011-01-06
通讯作者: 张海燕

Selecting human fetal hepatic progenitor cells based on α-fetoprotein promoter activities

1.Department of Cell Biology, Municipal Laboratory for Liver Protection and Regulation of Regeneration, Capital Medical University, Beijing 100069, China; 2.Liver Diseases Research Center, Beijing Friendship Hospital, Capital Medical University, Beijing 100050, China

Received:2010-01-29 Revised:2010-06-02 Online:2011-01-06
Contact: ZHANG Hai-yan

摘要/Abstract

关键词: 肝脏前体细胞, 细胞克隆, 甲胎蛋白, 启动子, 免疫荧光

Abstract: Objective To select hepatic progenitor cell clones from human fetal liver cells (FLCs) based on α-fetoprotein (AFP) promoter activities. Methods AFP promoter was amplified from human fetal liver genome by polymerase chain reaction (PCR) and cloned into pGL3-basic vector, forming the pGL3-AFP in a direct orientation for the promoters to drive firefly luciferase expression. To analyze the specificity of the AFP promoter, the pGL3-AFP and pRL-TK plasmids were co-transfected into HepG2, A549, and HeLa cells; the latter two cells do not express AFP. In order to obtain the homogenous cell populations, the proliferating colonies were isolated from clonal cultures of FLCs, and the AFP promoter activity of each clone was analyzed in each well of the cell lysates after co-transfection of pGL3AFP and pRL-TK plasmids for 48hours. Immunofluorescence was used to confirm the AFP expression in each clone. Results The results of PCR, restriction enzyme cutting and DNA sequencing confirmed that the pGL3-AFP had been constructed successfully. After co-transfection of the pGL3-AFP and pRL-TK plasmids, the AFP promoter activity was detected in HepG2 cells, but was weakly detected in A549 and HeLa cells, indicating that the AFP promoter could drive downstream firefly luciferase gene expression in AFP-expressing cells. Although the promoter activity in FLCs was lower than that in HepG2 cells, it was higher than that in AFP-non-expressing A549 and HeLa cells, further indicating that there were AFP-expressing cells among the FLCs. Five proliferating cell colonies were generated from clonal cultures of the FLCs, and the AFP promoter activity could be detected in one of the colonies. Immunofluorescence results revealed that the percentage of AFP positive cells was (99.1±0.6)% in this clone, indicating a hepatic progenitor cells clone. Conclusion The homogenous hepatic progenitor cell clones could be selected by AFP promot

Key words: Hepatic progenitor cell, Cell clone, α-fetoprotein, Promoter, Immunofluorescence

中图分类号:

R329.2

王萍;刘保清 ;李卫红;董凌月;尤红;贾继东;安威;张海燕. 利用甲胎蛋白启动子活力筛选人胚胎肝脏前体细胞[J]. , 2011, 42(1): 45-49.

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利用甲胎蛋白启动子活力筛选人胚胎肝脏前体细胞

Selecting human fetal hepatic progenitor cells based on α-fetoprotein promoter activities

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