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作 者:冯龙[1,2] 郭文涛[3] 路武豪[4] 孙萨迦[2] 董子明[2]
机构地区:[1]河南中医学院基础医学院,河南郑州450008 [2]郑州大学基础医学院,河南郑州450001 [3]漯河医学高等专科学校,河南漯河462002 [4]郑州大学第一附属医院,河南郑州450052
出 处:《肿瘤基础与临床》2014年第3期185-189,共5页journal of basic and clinical oncology
基 金:国家自然科学基金资助项目(编号:30471952)
摘 要:目的构建食管癌细胞Eca9706 DNA聚合酶β(DNA polβ)基因敲除载体,为DNA polβ基因敲除奠定基础。方法应用体细胞基因敲除技术的方法和原理,根据DNA polβ基因序列,设计并合成2对特异性引物(UP1/UP2和DOWN1/DOWN2),通过PCR扩增获得上游同源序列(UP)和下游同源序列(DOWN),其中上游同源序列长1 268 bp,下游同源序列长2 150 bp,将其插入骨架载体pcDNA3.1,从而构建了DNA polβ基因敲除载体pOUT-polβ,最后用PCR、酶切和测序进行鉴定。结果经过PCR筛选,限制性酶切及DNA测序鉴定,证实上游同源序列(UP)和下游同源序列(DOWN)2个片段插入正确。结论通过本研究所述方法,成功构建了用于食管癌细胞Eca9706 DNA polβ基因敲除载体pOUT-polβ。Objective To construct Eca9706 cell DNA polymerase 13 (DNA polβ) gene targeting vector. Meth- ods According to the principle of somatic gene targeting and DNA polβ sequence, the two special primers were de- signed and synthesized( UP1/UP2 and DOWN1/DOWN2)to amplify the up homologous sequence and the down ho- mologous sequence. The up sequence(1 268 bp) and the down sequence(2 150 bp) were inserted into skeleton vector pcDNA3.1, then DNA polβ gene targeting vector pOUT-polβ was constructed. Finally, the targeting vector was identified by PCR, restriction enzyme digestion and sequencing. Results The up sequence and the down se- quence were exactly inserted into skeleton vector pcDNA3.1, then DNA poll3 gene targeting vector pOUT-polβ was constructed. Conclusion The Eca9706 cell DNA polβ gene targeting vector was established successfully by using the method in this thesis.
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