人snail真核表达载体构建与鉴定  

Construction and Identification of Human Snail Gene Eukaryotic Vector

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作  者:杨乐[1] 郭晓波[2] 陈洪志[1] 成健[3] 董济民[1] 丁海霞[1] 王冠杰[1] 

机构地区:[1]西安交通大学附属西安市中心医院肿瘤科,陕西西安710000 [2]西安交通大学附属西安市中心医院血液科,陕西西安710000 [3]西安交通大学附属西安市中心医院妇产科,陕西西安710000

出  处:《现代生物医学进展》2017年第3期410-413,共4页Progress in Modern Biomedicine

基  金:陕西省自然科学基础研究计划项目(2014JM2-8182)

摘  要:目的:构建人snail基因真核表达载体并鉴定。方法:使用RT-PCR法获取人snail基因全长c DNA,经Bam H I、Eco R I双酶切、连接,插入pc DNA3.1(+)真核表达载体,转化TOP10感受态细胞,用含氨苄青霉素的LB培养基筛选阳性克隆,提取质粒双酶切电泳及测序鉴定,瞬时转染siha细胞Western-blot从蛋白水平鉴定重组质粒在真核细胞内的表达。结果:pc DNA3.1-snail重组质粒经酶切电泳符合预期片段,测序鉴定插入片段与NCBI Gen Bank文库中人snail序列一致,重组质粒瞬时转染后snail蛋白表达量明显增高。结论:成功构建pc DNA3.1-snail重组质粒载体,为进一步探讨snail基因生物学功能奠定了基础。Objective: To establish pc DNA3.1-snail eukaryotic recombinant expression plasmid. Methods: Human Snail gene c DNA was amplified by reverse transcription polymerase chain reaction(RT-PCR). After digested by Bam H I,Eco R I and ligation,Snail was inserted into pc DNA3. 1(+)eukaryotic expression vector. The positive colonies were screened and identified by single,double enzyme digest,agarose gel electrophoresis and DNA sequence analysis. pc DNA3. 1-snail plasmid was then transfected into siha cell line with Turbo Fect Transfection Reagent. Western-blot was used to detect the protein expression of snail. Results: The pc DNA3.1-snail recombinant plasmid was verified by enzyme digestion electrophoresis showed the expected fragment. The inserted sequence in pc DNA3.1(+)-snail was the same as the sequence of snail c DNA published in NCBI Gen Bank. Western blot results validated the recombinant plasmid expressed in siha cell line efficiently. Conclusion: The eukaryotic recombinant expression plasmid of pc DNA3.1(+)-snail was successfully constructed.

关 键 词:SNAIL 重组质粒 载体构建 

分 类 号:R-33[医药卫生] Q78[生物学—分子生物学]

 

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