Objective To construct and identify an eukaryotic expression vector of siRNA-inhibited CDC25A expression in mammalian cells.Methods CDC25A-specific siRNA was designed and synthesized according to the sequence of CDC25A.After annealing the nucleic acid fragment of the siRNA to form the double-stranded, they were connected with the eukaryotic expression vector psilencer4.1 which was pre-digested with Bam HI and Hind III.Then the constructed vectors, named psilencer4.1-CDC25A and psilencer4.1-Control, were digested and sequenced.Results The vector of siRNA-inhibited CDC25A expression and the negative control vector were constructed, sequenced and identified.Conclusion The successful construction and validation of the siRNA-inhibited CDC25A expression vector lays a good foundation for the next steps in CDC25A-related study.%目的 在哺乳动物细胞中构建并鉴定抑制CDC25A表达的siRNA真核表达载体.方法 根据CDC25A的基因序列,设计特异性的siRNA,将合成的siRNA 核酸片段退火形成双链后连接到经Bam HI和HindⅢ双酶切后的psilencer4.1真核表达载体,命名为psilencer4.1-CDC25A以及psilencer4.1-Control,并进行酶切及测序鉴定.结果 通过酶切鉴定和序列测定,成功地构建出抑制CDC25A表达的siRNA载体及其阴性对照载体.结论 成功构建和验证了siRNA真核表达载体,为下一步研究奠定了良好的基础.
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