应用抑制性消减杂交技术克隆和筛选PS1TP5反式激活相关基因

目的构建乙型肝炎病毒前-S1蛋白反式激活基因5(PS1TP5)的反式激活相关基因差异表达的cDNA,克隆PS1TP5蛋白反式激活相关基因。方法以PS1TP5表达质粒pcDNA3.1(-)-myc-his(A)-PS1TP5转染HepG2细胞,以空载体pcDNA3.1(-)-myc-his(A)为对照,制备转染后的细胞裂解液,提取mRNA并合成cDNA,经RsaⅠ酶切后将实验组cDNA分成两组,分别衔接两种不同接头,再与对照组cDNA进行两次消减杂交及两次PCR反应,产物与T/A克隆载体连接,构建cDNA消减文库,并转染大肠杆菌进行文库扩增,随机挑选克隆经PCR鉴定后进行测序及同源性分析。结果成功构建人PS1TP5蛋白反式激活相关基因差异表达的cDNA。扩增后得到70个200～1 000 bp插入片段的克隆,随机挑选其中30个插入片段测序,并通过生物信息学分析获得其全长基因序列,结果共获得24种编码基因,其中1个为未知功能的新基因,电子拼接后命名为HBV PS1TP5TP1(乙型肝炎病毒前-S1蛋白反式激活蛋白5反式激活蛋白1),GenBank注册号DQ487761。结论筛选到的cDNA全长序列,包括一些与细胞...

Screening and cloning of the PS1TP5 transactivation related genes by suppression subtractive hybridization

Objective To clone and identify human genes PS1TP5 transactivation related genes by constructing a cDNA subtractive library with suppression subtractive hybridization(SSH). Methods Suppression subtractive hybridization and bioinformatics technique were used for screening and cloning the target genes transactivated by PS1TP5 protein.The mRNA was isolated from HepG2 cells transfected pcDNA3.1(-)-myc-his(A)-PS1TP5 and pcDNA3.1(-)-myc-his(A) empty vector,respectively,and SSH method was employed to analyze the d...