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β雌激素受体沉寂表达载体的构建及表达
引用本文:孙旭妍,陶敏芳,程蔚蔚,王玉东. β雌激素受体沉寂表达载体的构建及表达[J]. 中国医药生物技术, 2010, 5(5): 353-356. DOI: 10.3969/cmba.j.issn.1673-713X.2010.05.005
作者姓名:孙旭妍  陶敏芳  程蔚蔚  王玉东
作者单位:1. 上海交通大学附属第六人民医院妇产科,200233
2. 上海交通大学附属国际和平妇幼保健院,200030
3. 200233,上海交通大学附属第六人民医院妇产科;200030,上海交通大学附属国际和平妇幼保健院
基金项目:国家自然科学基金,上海市科委"创新行动计划"重大基础研究项目子课题,上海市卫生局基金,上海市卫生局青年基金 
摘    要:目的构建雌激素受体β(ERβ)亚型沉寂表达载体,并观察其转染成骨细胞后抑制ERβ基因表达的效果。方法参考人ERβ基因mRNA序列,设计、合成ERβ-shRNA的DNA Oligo后行PCR扩增,获得的shRNA双链DNA片段与pLVTHM-GFP质粒双酶切后连接,转化大肠杆菌E.coliDH5α感受态细胞。取鉴定正确的pLVTHM-GFP/ERβ-shRNA重组质粒转染人成骨hMG63细胞,实验分空白载体组、空白对照组和ERβ-siRNA组,转染48h后于倒置荧光显微镜下观察各组细胞的转染效果,并采用流式细胞术检测转染效率。抽提各组细胞的总RNA,经RT-PCR生成cDNA,Realtime-PCR检测ERβ基因的抑制效率。结果倒置荧光显微镜下观察显示,ERβ-siRNA组hMG63细胞90%以上呈现绿色荧光。流式细胞术检测ERβ-shRNA转染hMG63细胞的转染效率为92.3%。Realtime-PCR检测结果表明,ERβ-siRNA组ERβ表达量(0.17±0.01)仅约为空白载体组(1.00±0.01)的17.3%(P0.001),ERβ-siRNA对hMG63细胞ERβ基因的抑制效率约为83%。结论成功建立了人ERβ沉寂表达的成骨细胞模型,慢病毒载体介导的ERβ-siRNA能有效抑制成骨细胞ERβ基因的表达,满足了研究成骨细胞中ERβ相关功能的需要。

关 键 词:成骨细胞  RNA,小分子干扰  雌激素受体β
收稿时间:2010-07-29

Construction and expression of silence expression vector for beta-estrogen receptor
SUN Xu-yan,TAO Min-fang,CHENG Wei-wei,WANG Yu-dong. Construction and expression of silence expression vector for beta-estrogen receptor[J]. Chinese Medicinal Biotechnology, 2010, 5(5): 353-356. DOI: 10.3969/cmba.j.issn.1673-713X.2010.05.005
Authors:SUN Xu-yan  TAO Min-fang  CHENG Wei-wei  WANG Yu-dong
Affiliation:Author ( Department of Obstetrics and Gynecology, the 6th People's Hospital, Shanghai Jiaotong University, Shanghai 200233, China ; International Peace Maternal and Child Health Hospital, Shanghai Jiaotong University, Shanghai 200030, China )
Abstract:Objective To construct silence expression vector for beta-estrogen receptor (ERβ), and evaluate the inhibition efficiency of ERD in hMG63 cells.Methods According to the mRNA sequence of human estrogen receptor beta (ERβ),the DNA Oligo of ERβ-shRNA was designed, synthesized, PCR amplification and inserted into the vector of pLVTHM-GFP, which was integrated into the expression plasmid of pLVTHM-GFP/ERβ-shRNA. After correctly identified from the competent cell of E. coli DH5α, the pLVTHM-GFP/ERβ-shRNA finally was transfected into hMG63 cells. The transfection efficiency was evaluated by the inverted fluorescence microscope and flow cytometry for ERβ-siRNA group, blank vector group and control group. The inhibition efficiency of ERβ gene was determined by Realtime-PCR.Results Inverted fluorescence microscope showed that 90% of hMG63 cells in the ERβ-siRNA group appeared green fluorecent. The transfection efficiency measured by FCM for hMG63 cells transfected with ERβ-shRNA was 92.3%. The relative expression value of ERβ-siRNA group (0.17 ± 0.01) was 17.3% of the blank vector group (1.00 ± 0.01) (P 〈 0.001). The inhibition efficiency of ERβ-siRNA for ERβ gene in the hMG63 cells was 83%.Conclusion The cell model of ERβ silence was successfully developed in hMG63 cells. Lentiviral vector-mediated ERβ-siRNA could effectively inhibit the expression of ERβ in hMG63 cells, which meets the research for ERβ function in hMG63 cells.
Keywords:RNA
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