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作 者:李敏[1] 郝林琳[1] 刘松财[1] 张永亮[2]
机构地区:[1]吉林大学畜牧兽医学院,长春130062 [2]华南农业大学,广州510095
出 处:《现代生物医学进展》2008年第3期421-423,共3页Progress in Modern Biomedicine
基 金:国家自然科学基金资助(编号:30571355)
摘 要:目的:设计并合成生长抑素受体SSTR5基因siRNA序列,并构建其短发夹shRNA慢病毒表达质粒。方法:以小鼠SSTR5基因为靶序列,用在线软件分析、设计并合成其有效siRNA,退火形成双链DNA后,与经BamHⅠ和EcoRⅠ双酶切线性化慢病毒表达载体pSHR-Pμzro/GFP连接,产生pLV-shSSTR5重组慢病毒质粒,将重组质粒转化大肠杆菌DH 5α感受态细胞,PCR筛选阳性克隆,测序鉴定。结果:构建的重组表达质粒PCR产物为161bp,其中插入的SSTR5-siRNA片段为61bp,测序结果与参考序列完全一致。结论:成功构建了小鼠SSTR5基因特异性shRNA慢病毒表达质粒。Objective: To design and construct siRNA lentiviral expression plasmid targeting mo use SSTR5 (somatostatin receptor) gene by RNA interfering technique. Methods: According to mouse SSTR5 gene deposited in Genbank, the oligo primers targeting mouse SSTR5 gene were designed and synthesized. The PCR product was cloned into linear pSHR-Pμro/GFP by BamH I and EcoR in order to construct a siRNA expression plasmid. Results: The PCR product of constructed plasmids was 161bp, in which, inserted SSTR5-siRNA flagment was 61bp, and DNA sequencing demonstrated that the inserted fragrnents were consistent with the reference sequences. Conclusion: The lentivirus RNAi vector of SSTR5 was constructed successfully, which provides a tool for further study in the effects of SSTR5 gene expression on mouse growth with RNAi technology.
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