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机构地区:[1]广州中医药大学第二临床医学院,广东广州510405 [2]中国科学院广州生物医药与健康研究院,广东广州510530 [3]广州中医药大学广东省中医院检验医学部,广东广州510370
出 处:《实验技术与管理》2018年第2期62-66,共5页Experimental Technology and Management
基 金:国家自然科学基金项目(81602608)
摘 要:将重组质粒转化到大肠杆菌BL21(DE3)中,在不同的诱导时机、诱导温度、IPTG的浓度和Mg^(2+)浓度条件下培养大肠杆菌,通过SDS-PAGE和发光强度检测分析TAT-LUC的酶活性强度及表达量;将高活性的TAT-LUC与LUC对比检测ATP,通过发光强度分析TAT-LUC的敏感性和可靠性。表明:在含Mg^(2+)浓度为50mmol/L的LB培养基中将大肠杆菌培养至OD600为0.6时,加入终浓度为0.5mmol/L的IPTG,22℃诱导16h可获得大量高活性的TAT-LUC;相比LUC,TAT-LUC可以检测到小于10nmol/L的ATP,发光强度与ATP含量呈强相关性(R2=0.99);并且不用裂解细胞,TAT-LUC可直接检测至少40个细胞内ATP;穿膜肽标记的荧光素酶蛋白成功用于检测活细胞内的ATP含量。The recombinant plasmid is transformed into Escherichia coli BL21(DE3),and Escherichia coli is cultivated under the conditions of different induction time,induction temperature,concentration of IPTG and Mg(2+) concentration.Through SDS-PAGE and luminescence intensity detection,the enzyme activity intensity and expression of TAT-LUC are analyzed.The high active TAT-LUC is compared with LUC to detect ATP,and through the luminous intensity,the sensitivity and reliability of TAT-LUC are analyzed.The results show that when the Escherichia coli in an LB medium with the concentration of Mg(2+) which is 50 mmol/L is cultivated from OD600 to 0.6,IPTG with a final concentration of0.5 mmol/L is added and a large amount of the highly active TAT-LUC can be obtained after the 16 hinduction at 22℃.In comparison with LUC,TAT-LUC can detect ATP of less than 10 nmol/L,and the intensity of luminescence is strongly correlated with the content of ATP(R2=0.99).Without cracking cells,TAT-LUC can directly detect at least40 intracellular ATPs.The luciferase protein labeled by membrane peptide has been successfully used to detect the content of ATP in living cells.
分 类 号:TP212.3[自动化与计算机技术—检测技术与自动化装置]
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