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作 者:黄思斯[1,2] 焦杨 谢萍[2] 王青[2] 张令强[1,2]
机构地区:[1]中南大学生物科学与技术学院,长沙410013 [2]军事医学科学院放射与辐射医学研究所,北京100850 [3]陕西武警总队医院碎石中心,西安710054
出 处:《军事医学》2012年第7期520-523,共4页Military Medical Sciences
基 金:国家重大科学研究计划项目(2007CB914601);国家杰出青年科学基金(31125010)
摘 要:目的为了鉴定并验证CUL4A-DDB1泛素连接酶复合体中参与DNA损伤修复反应过程的1~2种关键成分在损伤识别、早期及晚期修复中的动态变化,拟构建含有串联亲和纯化(TAP)标签载体并筛选高表达CUL4A/DDB1的细胞株,建立DNA双链断裂模型。方法利用PCR获得CUL4A/DDB1基因,构建重组表达载体pNTAP-A-CUL4A/DDB1;使用顺铂和电离辐射刺激等外界刺激建立合适的DNA双链断裂细胞模型,使用G418筛选稳定表达CUL4A/DDB1的细胞株。结果与结论成功构建pNTAP-A-CUL4A/DDB1表达载体,建立合适的DNA双链断裂细胞模型,筛选得到稳定表达CUL4A/DDB1的细胞稳定株,为下一步质谱分析CUL4A-DDB1泛素连接酶在DNA损伤修复过程中的新功能打下基础。Objective To find the dynamic change of one or more key components of the CUL4A-DDB1 complex involved in the process of DNA damage and repair and to construct tandem affinity purification(TAP) targeted plasmids of CUL4A/DDB1 and cell models responding to DNA damage. Methods The full-length gene of CUL4A/ DDB1 by PCR was used to express the recombinant expression vector pNTAP-A-CUL4A/DDB1. Exposure to eisplatin, irradiation and other cellular stresses was performed to select appropriate cell models responding to DNA damage. After the G418 resistant cells were induced, CUIAA/DDB1 activity of the supernatant was determined. Results and Conclusion The CUIAA and DDB1 genes by PCR were amplifid and then recombined into the pNTAP-A expression vector. Appropriate cell models responding to DNA damage were successfully selected arid cell lines that stably express CUL4A/DDB1 were obtained. These lines can be used formass chromatography to analyze the functional role of CUL4A-DDB1 E3 ligase in DNA damage and repair.
关 键 词:DNA损伤 CUL4A-DDB1 串联亲和纯化
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