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作 者:白元松[1] 陈玉丙[2] 石张镇[1] 卢振霞[1]
机构地区:[1]吉林大学中日联谊医院血液肿瘤科,吉林长春130031 [2]吉林大学第二医院放疗科
出 处:《中华血液学杂志》2008年第6期393-396,共4页Chinese Journal of Hematology
基 金:基金项目:国家自然科学基金(30672425)
摘 要:目的研究慢病毒载体(1entivirus vector)基因转导技术对脐血CD34^+细胞基因表达的影响。方法将携带绿色荧光蛋白(GFP)基因的第三代自身失活(self-inactivating,SIN)慢病毒载体导入CD34^+细胞。提取被病毒感染细胞的总RNA,应用cDNA微阵列技术对慢病毒载体感染的脐血CD34’细胞及正常对照细胞进行差异基因表达谱分析。结果在23000个被检测基因中,与无基因导入的对照组细胞比较,基因导入细胞中表达的上调基因共2个,分别为IGSF4和HEC基因,下调基因共6个,分别为HNRPA0、ZNF205、FLNA、CLK3、LDB1、ACTA1。进一步对筛选出的差异表达基因进行半定量RT-PCR分析证实基因表达水平变化不明显。结论本实验中应用的慢病毒载体对脐血CD34^+细胞基因表达无明显影响,有望成为临床基因治疗有效且安全的工具。Objective To investigate the influence of gene transduction mediated by lentivims vector on haman CD34^+ cord blood cell (CBCs) gene expression. Methods CD34^+ cells were isolated and trans- duced with the third-generation self-inactivating (SIN) lentiviral vector carrying green fluorescent protein (GFP). The total RNA from transduced cells was extracted and the differences of genotypes between the transduced and non-transduced CD34^+ cells were determined with cDNA microarray analysis . Results In 23000 genes two were upregulated and six downregulated. These changes were not confirmed by semi-quanti-tative RT-PCR method. Conclusions Lentiviral vector used in this study do not influence significantly on the gene expression of CD34^+ CBCs, and the vector system may be a useful and safe one in clinical gene therapy.
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