Avian influenza virus(AIV) nonstructural 1(NS1) gene was amplified by real-time polymerse chain reac tion(RT-PCR) and inserted into pET28a, then transformed into E. coli BL21(DE3) competent cell. With the indu...Avian influenza virus(AIV) nonstructural 1(NS1) gene was amplified by real-time polymerse chain reac tion(RT-PCR) and inserted into pET28a, then transformed into E. coli BL21(DE3) competent cell. With the induction of isopropyl-β-D-thiogalactoside(IPTG) and the purification of Ni-NTA column, we finally obtained purified NS1 protein. T7-phage display system was used to screen the proteins that interacted with NS1 from lung cell cDNA li brary. The selected positive clones were identified by DNA sequencing and analyzed by BLAST program in Gene Bank. Two proteins were obtained as NS1 binding proteins, Homo sapiens nucleolar and coiled-body phosphoprotein 1(NOLC1) and Homo sapiens similar to colon cancer-associated antigen. By co-immunoprecipitation and other me thods, Homo sapiens NOLC1 was found to interact with the NS1 protein, the results would provide the basis for fur ther studying biological function of NS1 protein.展开更多
目的:用T7噬菌体筛选系统筛选乙型肝炎病毒PreS1的相互作用蛋白。方法:应用T7噬菌体展示技术,以通过原核表达的方式得到的乙型肝炎病毒PreS1作为靶分子,对噬菌体人肝细胞cDNA文库进行生物筛选,对筛选到的克隆进行DNA序列分析及同源性搜...目的:用T7噬菌体筛选系统筛选乙型肝炎病毒PreS1的相互作用蛋白。方法:应用T7噬菌体展示技术,以通过原核表达的方式得到的乙型肝炎病毒PreS1作为靶分子,对噬菌体人肝细胞cDNA文库进行生物筛选,对筛选到的克隆进行DNA序列分析及同源性搜索。结果:经鉴定得到1个阳性克隆,确定了能与乙型肝炎病毒PreS1相互作用的蛋白可能为:细胞色素C氧化酶1(Cytochrome c Oxidase Subunit I,COX1)。结论:T7噬菌体展示筛选系统是筛选相互作用蛋白的一种简单、快速和有效的手段,筛选到的相互作用蛋白为进一步探讨PreS1的致病机制提供重要依据。展开更多
从T7噬菌体培养液中粗提噬菌体颗粒,经热裂解后用苯酚、氯仿抽提进而获得纯净的T7噬菌体DNA。用PCR、酶切法鉴定T7噬菌体DNA的完整性。通过对不同感受态细菌浓度、T7噬菌体DNA用量、电转化电压条件的优化,建立了T7噬菌体反向遗传拯救方...从T7噬菌体培养液中粗提噬菌体颗粒,经热裂解后用苯酚、氯仿抽提进而获得纯净的T7噬菌体DNA。用PCR、酶切法鉴定T7噬菌体DNA的完整性。通过对不同感受态细菌浓度、T7噬菌体DNA用量、电转化电压条件的优化,建立了T7噬菌体反向遗传拯救方法。结果显示,提取的DNA结构完整,能够被特异性酶切割,多克隆位点序列正确。T7噬菌体的反向遗传拯救方法最优化条件为200 ng T7噬菌体DNA、1 ml 5×109感受态细菌、1.5 kV电转化电压,在此条件下获得的拯救效率为3.5×105 PFU/ng(DNA)。展开更多
基金Supported by the National Natural Science Foundation of China(No.30671852)the Open Research Fund Program of the State Key Laboratory of Virology of China(Nos.2010009, 2007007) the Research Fund of the Key Laboratory of Department of Education of Liaoning Province, China(No.2009S043)
文摘Avian influenza virus(AIV) nonstructural 1(NS1) gene was amplified by real-time polymerse chain reac tion(RT-PCR) and inserted into pET28a, then transformed into E. coli BL21(DE3) competent cell. With the induction of isopropyl-β-D-thiogalactoside(IPTG) and the purification of Ni-NTA column, we finally obtained purified NS1 protein. T7-phage display system was used to screen the proteins that interacted with NS1 from lung cell cDNA li brary. The selected positive clones were identified by DNA sequencing and analyzed by BLAST program in Gene Bank. Two proteins were obtained as NS1 binding proteins, Homo sapiens nucleolar and coiled-body phosphoprotein 1(NOLC1) and Homo sapiens similar to colon cancer-associated antigen. By co-immunoprecipitation and other me thods, Homo sapiens NOLC1 was found to interact with the NS1 protein, the results would provide the basis for fur ther studying biological function of NS1 protein.
文摘目的:用T7噬菌体筛选系统筛选乙型肝炎病毒PreS1的相互作用蛋白。方法:应用T7噬菌体展示技术,以通过原核表达的方式得到的乙型肝炎病毒PreS1作为靶分子,对噬菌体人肝细胞cDNA文库进行生物筛选,对筛选到的克隆进行DNA序列分析及同源性搜索。结果:经鉴定得到1个阳性克隆,确定了能与乙型肝炎病毒PreS1相互作用的蛋白可能为:细胞色素C氧化酶1(Cytochrome c Oxidase Subunit I,COX1)。结论:T7噬菌体展示筛选系统是筛选相互作用蛋白的一种简单、快速和有效的手段,筛选到的相互作用蛋白为进一步探讨PreS1的致病机制提供重要依据。
文摘从T7噬菌体培养液中粗提噬菌体颗粒,经热裂解后用苯酚、氯仿抽提进而获得纯净的T7噬菌体DNA。用PCR、酶切法鉴定T7噬菌体DNA的完整性。通过对不同感受态细菌浓度、T7噬菌体DNA用量、电转化电压条件的优化,建立了T7噬菌体反向遗传拯救方法。结果显示,提取的DNA结构完整,能够被特异性酶切割,多克隆位点序列正确。T7噬菌体的反向遗传拯救方法最优化条件为200 ng T7噬菌体DNA、1 ml 5×109感受态细菌、1.5 kV电转化电压,在此条件下获得的拯救效率为3.5×105 PFU/ng(DNA)。