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机构地区:[1]潍坊学院生物工程学院,中国山东潍坊261061 [2]潍坊医学院细胞生物学教研室,中国山东潍坊261042
出 处:《生命科学研究》2009年第1期55-59,共5页Life Science Research
基 金:山东省自然科学基金资助项目(Y2007079);潍坊市科技发展计划项目(2007028)
摘 要:为了得到超量表达胶质细胞源神经营养因子(glial cell line-derived neuotrophic factor,GDNF)的NIH-3T3细胞株,用于制作精原干细胞(spermatogonial stem cells,SSCs)培养的饲养层,通过RT-PCR方法成功地从幼年小鼠睾丸中克隆了gdnf基因,构建了真核表达载体pcDNA3.1-gdnf,并用其转染NIH-3T3细胞.对筛选出的阳性细胞克隆进行的免疫荧光染色、RT-PCR和Western blotting的结果表明,获得了超量表达gdnf基因的NIH-3T3细胞株,这为精原干细胞的培养奠定了基础.In order to obtain the feeder cells expressing the glial cell line-derived neurotrophic factor (GDNF) to culture spermatogonial stem cells (SSCs), the gdnf gene from the testes of normal immature mice was cloned by RT-PCR method, the eukaryotic expression vector of pcDNA3. 1-gdnf was constructed and then transfected into NIH-3T3 cells. Sequence analysis identified that 723 bp eDNA of gdnf was obtained precisely, and the transgenetie over-expression were also demonstrated with immunofluorescence detection, RT-PCR and Western blotting. Thus, the NIH-3T3 feeders over-expressing gdnf was obtained successfully and the basis of SSCs culture was established.
关 键 词:GDNF RT-PCR NIH-3T3 基因表达
分 类 号:R742.5[医药卫生—神经病学与精神病学]
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