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作 者:王义生[1] 张弛[1] 李月白[2] 赵国强[3] 王少华[1] 李振伟[1] 殷力[1] 刘宏建[1]
机构地区:[1]郑州大学第一附属医院骨科,河南省高等学校临床医学重点学科开放实验室,郑州450052 [2]郑州大学基础医学院生物化学教研室,郑州450001 [3]郑州大学基础医学院微生物学与免疫学教研室,郑州450001
出 处:《郑州大学学报(医学版)》2008年第3期477-479,共3页Journal of Zhengzhou University(Medical Sciences)
基 金:国家自然科学基金资助项目30672128
摘 要:目的:构建针对过氧化物酶体增殖子活化受体-γ(PPARγ)基因的siRNA腺病毒载体。方法:依据siR-NA设计原则,在PPARγmRNA(AF013266)序列中设计2个特异性靶序列(36-54、73-91),体外合成对应发卡样DNAs,退火后先将其克隆入pSIREN-Shuttle载体,再亚克隆入pAdeno腺病毒载体,对插入序列进行DNA序列分析。结果:发卡样siRNA单链DNA寡核苷酸退火后,电泳可见明亮靶条带。连接退火寡核苷酸和pSIREN-Shuttle载体得到阳性克隆pSIREN-Shuttle-siPPARγ-36、pSIREN-Shuttle-siPPARγ-73。同源重组后得到亚克隆pAdeno-siPPARγ-36、pAdeno-siPPARγ-73,测序证实插入序列与设计序列完全一致。结论:成功构建2个靶向PPARγ基因的siRNA载体pAdeno-siPPARγ-36和pAdeno-siPPARγ-73。Aim: To construct the siRNA adenovirus vector targeting peroxisome proliferator-activated receptor-γ (PPARγ). Methods:Two specificity target sequences( 36-54.73-91 from PPARγ mRNA sequencer AF013266 were designed according to the principle of design on siRNA, then the corresponding hairpin-shaped DNA fragment was synthesized in vitro. The product was cloned into pSIREN-Shuttle vector after annealing,then subeloned into siRNA adenovirus vector pAdeno. The insertion DNA sequences were analyzed. Results : The hairpin-shaped siRNA single strand DNA oligonucleotide showed an obvious electrophoresis strip after annealing. The positive clones pSIREN-Shuttle-siPPARγ-36 and pSIREN-Shuttle-siPPARγ-73 were obtained by connecting the annealed oligonucleotide with pSIREN-Shuttle vector. Positive subclone pAdeno-siPPARγ-36 and pAdeno-siPPARγ-73 were obtained by homologous recombination. The inserted sequences were confirmed by sequencing. Conclusion: Two siRNA adenovirus vector targeting PPARγ,pAdeno-siPPARγ-36 and pAdeno-siPPARγ-73, are successfully constructed.
关 键 词:RNA干扰 过氧化物酶体增殖子活化受体-γ 腺病毒载体 克隆
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