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作 者:刘超[1] 汤斌[1] 曾杨[1] 于美娟[1] 石奕武[1] 廖卫平[1]
机构地区:[1]广州医学院第二附属医院神经科学研究所,510260
出 处:《实用医学杂志》2011年第11期1908-1910,共3页The Journal of Practical Medicine
基 金:国家自然科学基金资助项目(编号:30900451);广东省自然科学基金资助项目(编号:10151018201000021)
摘 要:目的:构建Ⅰ型钠通道(NaV1.1)与红色荧光蛋白(DsRed)共表达载体及其突变载体。方法:利用In-Fusion技术将SCN1A基因亚克隆到DsRed真核细胞表达载体(pCMV-IRES-DsRed)。限制性内切酶对载体进行酶切并回收线性载体片段,PCR扩增SCN1A基因(与线性载体对应两端有15个相同碱基),In-Fusion技术进行融合即得到pCMV-SCN1A-IRES-DsRed。将其转染HEK293T细胞,Western blot检测NaV1.1的表达。定点诱变试剂盒对其进行定点诱变。结果:成功构建NaV1.1与DsRed共表达载体,SCN1A基因所编码的第1623位密码子由谷氨酸(Glu)突变为丙氨酸(Ala)。结论:NaV1.1与DsRed共表达载体及其突变载体的构建成功,为进一步研究该突变位点导致NaV1.1功能的改变奠定了基础。Objective To construct the co-expression vector of Nay1.1 and DsRed, and the corresponding vector containg mutated Nav1.1. Methods pCMV-IRES-DsRed vector was digested by restriction enzymes and the lined vector was purified. SCN1A gene was performed from pCMV-SCN1A plasmid. SCN1A gene was cloned into the linearized pCMV-SCN1A-IRES-DsRed vector using In-Fusion technology. The corresponding mutational vector was prepared using site-directed mutagenesis kit. The recombinant plasmid was transformed into HEK293T cells using lipofectamine 2000. Nav1.1 expression in HEK293T cells was detected by western blotting assay. Results Co- expression vectors of DsRed and Nav1.1 or mutated Navl.1 were successfully constructed and the mutation site in SCN1A was EI623A. Conclusions The constructed co-expression vector of Nav1.1 and DsRed and its mutational plasmid containing SCNIA EI623A mutation may lay a good foundation for SCN1A function study.
关 键 词:钠通道 红色荧光蛋白 In.Fusion技术 诱变 SCN1A 癫痫
分 类 号:R742.1[医药卫生—神经病学与精神病学]
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