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作 者:张小云[1] 曹广义[1] 殷虹[1] 时兰英[1] 苏友强[1]
机构地区:[1]南京医科大学生殖医学国家重点实验室,江苏南京211166
出 处:《南京医科大学学报(自然科学版)》2017年第7期818-822,共5页Journal of Nanjing Medical University(Natural Sciences)
基 金:国家重大科学研究计划(2014CB943200;2013CB945500);国家自然科学基金面上项目(31471351;31271538);江苏省自然科学基金(BK20140061)
摘 要:目的:克隆小鼠的Marf1基因并使其在真核细胞HEK293T中异位表达,以研究MARF1蛋白在细胞中的表达和定位。方法:运用反转录-聚合酶链反应(reverse transcription-polymerase chain reaction,RT-PCR)扩增并获得Marf1基因编码序列,再利用新型分子克隆体系In-Fusion将该目的片段克隆至pCMV6-AC-3DDK和pCMV6-AN-m Kate两个真核表达载体中,由此所得融合质粒经限制性内切酶酶切电泳和测序筛选鉴定,将所得到的阳性质粒转染到HEK293T细胞中进行表达,然后利用DDK和m Kate标签抗体通过Western blot或免疫荧光的方法检测目的蛋白MARF1的表达和定位。结果:DNA测序鉴定证明Marf1基因克隆成功;Western blot检测到MARF1-3DDK和MARF1-m Kate融合蛋白在转染的HEK293T细胞内的表达;免疫荧光显示融合蛋白在转染后的HEK293T细胞质呈颗粒状分布,并与纺锤体共定位。结论:成功克隆了小鼠Marf1基因并实现了其在真核细胞HEK293T中的稳定表达,为进一步研究其功能和作用机制奠定了基础。Objective:To clone mouse Marfl gene and let it ectopically express in HEK293T cells,for studying its expression and mechanism. Methods:Marfl coding sequence was amplified by reverse transcription-polymerase chain reaction (RT-PCR)and was cloned into the eukaryotic cell-expression vector pCMV6-AC-3DDK and pCMV6-AN-mKate using the advanced In-Fusion cloning system. After verification by restriction digestion followed by electrophoresis and sequencing,the correctly cloned plasmid DNA was transfected into HEK293T cells. The expression of MARF1-3DDK and MARFI-mKate fusion protein in the transfected HEK293T cells was assessed by both Western blot and immunofluorescence using the antibodies against DDK and mKate tag proteins. Results: The correct cloning of Marfl was confirmed by restriction digestion and sequencing,and the expression of MARF1-3DDK and MARFI-mKate fusion protein was detected by Western blot. MARF1 fusion protein was detected to be localized either in the cyto- plasm in a punctate manner or on the mitotic spindles. Conclusion:Mouse Marfl gene was successfully cloned and expressed in HEK293T cells,which lays solid foundation for further studies on its functions and the related mechanisms.
关 键 词:Marf1 In-Fusion克隆 HEK293T
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