牛泡沫病毒（BSV）对牛免疫缺陷病毒（BIV）的激活作用

用瞬时表达分析等方法,证明牛泡沫病毒（ Ｂ Ｓ Ｖ）３０２６ 中国毒株能在体外激活牛免疫缺陷病毒（ Ｂ Ｉ Ｖ） 基因表达, Ｂ Ｓ Ｖ３０２６ 编码的反式激活因子 Ｂｏｒｆ１ 行使这种激活作用。缺失突变分析表明, Ｂｏｒｆ１ 在 Ｂ Ｉ Ｖ Ｌ Ｔ Ｒ 上靶序列位于－ ４１０／ － １１５（ ＋ １ 为转录起始位点） 区域,但其中的 Ｎ Ｆκ Ｂ 位点（ － ３６７／ － ３１９） 与这种激活作用无关,包括转录起点下游（ Ｒ Ｕ５ 区） 在内的－ １１５／ ＋ ２０４ 区域也与这种激活作用无关。该结果对研究 Ｂ Ｉ Ｖ 致病机理及防治 Ａ Ｉ Ｄ Ｓ 有重要意义。     

牛泡沫病毒内部启动子的克隆及功能分析

以该实验室分离并鉴定的牛泡沫病毒（ＢＦＶ３０２６）为材料,用ＰＣＲ方法首次克隆了位于ｅｎｖ基因３’端的内部启动了,经序列分析后,引入ｌｕｃ基因作瞬时分析。结果表明,该内部启动子不但基础活性高于ＬＴＲ,而且转录活怀在Ｔａｓ参与下被大大激活,其激活活性也远远高于ＬＴＲ。同源分析表明,非灵长类泡沫病毒内部启动子之间的同源性高于其与灵长类泡沫病毒内部妄动子之间的同源性。     

EB病毒胸苷激酶基因的定向克隆

采用异硫氰酸胍（ＧｕＳＣＮ）和硅藻从Ｂ９５－８细胞中快速抽摸板ＤＮＡ。根据ＥＢ病毒（ＥＢＶ）Ｂ９５－８株ＤＮＡ全序列及编码ＥＢＶ胸苷激酶（ＴＫ）的开放读框ＢＸＬＦ１的结构,设计合成一对引物,并在引物的５′一端分别引入ＥｃｏＲＩ和ＰｓｔＩ切点,用ＰＣＲ技术扩增出一含完整的ＥＢＶＴＫ基因的１．８４３ＫｂＤＮＡ片段,ＮｃｏＩ酶切分析鉴定,ＥｃｏＲＩ／ＰｓｔＩ双酶切ＰＣＲ产物和载体,使目的基因定向克隆至选     

HBV－DNA的PCR二步法扩增及其快速检测

ＨＢＶ－ＤＮＡ的ＰＣＲ二步法扩增及其快速检测方勤,吴云涛,蔡宜权（中国科学院武汉病毒研究所,武汉４３００７１）关键词ＨＢＶ－ＤＮＡ,二步温控ＰＣＲ,Ｓｏｕｔｈｅｒｎ杂交,生物素寡聚核苷酸杂交乙型肝炎是危害人类健康的主要疾病之一,其病原常用的检测方法多...     

马立克氏病病毒（MDV）814株B抗原基因的克隆及部分序列分析

提取感染鸡胚成纤维细胞ＭＤＶ－Ｉ弱毒株８１４病毒ＤＮＡ为模板,根据ＲＢＩＢ株ｇＢ基因５′及３′两端核苷酸离列设计引物,利用ＰＣＲ技术扩增了我国ＭＤＶ－Ｉ弱毒株８１４ｇＢ基因（２．９ｋｂ）将扩增片段平末端克隆到载体ｐＢｌｕｅｓｃｒｉｐｔＳＫ中ＥｃｏＲＶ位点,经ＢａｍＨＩ,ＨｉｎｄＩＩＩ酶切鉴定得到不同插入方向的重组质粒。构建圹增片段的酶切图谱及部分序列分析证明与ＲＢＩＢ株ｇＢ基因无差异,显示了极高的     

鸡传染性支气管炎病毒中国流行株免疫原S1基因的分子克隆、序列分析及其DNA免疫的初步研究

对来源于我国华东地区的鸡传染性支气管炎病毒流行株ＱＤ免疫原Ｓ１基因ｃＤＮＡ进行了克隆、序列分析和ＤＮＡ免疫的初步研究。ＲＴＰＣＲ扩增ＱＤ毒株的Ｓ１基因,将其５′和３′端分别进行分子修饰后插入克隆载体ｐＵＣ１８的ＢａｍＨⅠ／ＨｉｎｄⅢ位点,在大肠杆菌中实现了目的基因的克隆;利用英国ＩＢＶ毒株Ｓ１全基因核酸探针与ＱＤ毒株Ｓ１基因的重组克隆质粒分子杂交后,采用ＨａｅⅢ,ＰｖｕⅡ和ＸｂａⅠ等限制酶对此流行毒株Ｓ１基因ｃＤＮＡ进行了酶切分析;在测定ＱＤ毒株Ｓ１基因５′端高变区核苷酸序列并以此与ＩＢＶＭ４１,Ｈ１２０,６／８２及Ｂｅａｕｄ等参考毒株序列对比分析的基础上,构建了ＱＤ株Ｓ１基因ＤＮＡ免疫表达质粒,肌肉注射免疫小鼠后,鸡胚病毒中和试验的结果表明,ＩＢＶＳ１基因ＤＮＡ免疫表达质粒能诱导小鼠产生病毒特异的中和抗体,具有良好的免疫原性,初步显示基因疫苗在鸡传染性支气管炎防治上应用前景。     

犬细小病毒中国内蒙株VP2基因克隆及序列分析

从我国内蒙古地区流行的犬细小病毒病病犬的肠溶物中分离提纯犬细小病毒（ＣＰＶ）。提取病毒基因组ＤＮＡ,并以此ＤＮＡ为模板,采用人工合成的引物进行ＰＣＲ扩增,ＰＣＲ产物经ＢａｍＨＩ、ＳａｃＩ双酶切后,克隆于ｐＵＣ１９质粒的ＢａｍＨＩ／ＳａｃＩ位点。重组质粒ｐＵＣＶＰ２经ＰＣＲ鉴定、限制酶切分析和序列分析,结果表明：获得了犬细小病毒内蒙株（ＣＰＶ－ＩＭ）ＶＰ２基因的全长克隆,ＶＰ２基因全长１７５５ｎｔ,     

鸡传染性支气管炎病毒中国流行株免疫原S1基因的分子克隆,序？…

对来源于我国华东地区的鸡传染性支气管炎病毒流行株ＱＤ免疫原Ｓ１基因ｃＤＮＡ进行了克隆,序列分析了和ＤＮＡ免疫的初步研究,ＲＴ－ＰＣＲ扩增ＱＤ毒株的Ｓ１基因,将其５′和３′端分别进行了分子修饰后插入克隆载体ＰＵＣ１８的ＢａｍＨＩ／ＨｉｎｄⅢ位点,大肠杆菌中实现了目的基因的克隆,利用英国ＩＢＶ毒株Ｓ１全基因核酸探针与ＱＤ毒株Ｓ１基因的重组克隆质粒子分杂交后,采用ＨａｅⅢ,ＰｖｕⅡ和ＸｂａＩ等限制酶对此     

抗乙肝病毒表面抗原嵌合抗体基因在昆虫细胞中的表达

应用杆状病毒表达系统在昆虫细胞中表达了抗乙肝病毒表面抗原（ＨＢｓＡｇ）人－鼠嵌合抗体重,轻链基因,鼠源单克隆抗体ＯＨ３重,轻链可变区（ＶＨ,ＶＬ）ｃＤＮＡ分别与人免疫球蛋白恒区γ３,ｋ,ｃＤＮＡ拼接成人－鼠嵌合抗体基因,含嵌合抗体的转移载体与线性化病毒ＤＮＡ共转染Ｓｆ９细胞,并通过点杂交ＰＣＲ扩增和Ｓｏｕｔｈｅｒｎｂｌｏｔ分析获得重组病毒。Ｗｅｓｔｅｒｎｂｌｏｔ和竞争ＥＬＩＳＡ表明以重组病毒感染的     

水稻草矮病毒血清学和分子检测方法的比较

将间接ＥＬＩＳＡ、非放射性分子杂交和ＲＴ－ＰＣＲ三种方法应用于水稻草矮病毒（ＲＧＳＶ）的检测。结果表明,利用自制的融合蛋白ＧＳＴ－ＮＣ的抗血清检测ＲＧＳＶ的灵敏度为１ｍｇ鲜重的病株叶片或８４ｎｇ提纯病毒,利用地高辛（ＤＩＧ）标记的ＤＮＡ探针ＮＣ的点杂交方法检测ＲＧＳＶ的灵敏度为５０μｇ病叶或６ｎｇ病毒,而ＲＴ－ＰＣＲ的检测灵敏度则为１０μｇ病叶或２ｎｇ的病毒,对上述三种方法的灵敏度和可操作性也进行     

JDV与三种牛反转录病毒相互关系的初步研究

为研究JDV与其它三种牛反转录病毒BIV、BLV、BFV的相互作用关系,将以JDV、BIV、BLV、BFV的LTR为启动子,以Luc为报告基因的质粒和以上病毒反式激活因子的表达质粒共转染BLl2细胞系,通过瞬时表达分析试验证明了JDV和BIV的LTR和Tat之间亲缘关系很近,能够相互激活;JDV Tat可以反式激活BLVLTR,BLVTax不能激活JDVLTR;JDVLTR上存在BFVTas的应答元件;BLV、BFV和BIV的LTR和反式激活因子问不存在相互激活。     

JDV与三种牛反转录病毒相互关系的初步研究

为研究JDV与其它三种牛反转录病毒BIV、BLV、BFV的相互作用关系,将以JDV、BIV、BLV、BFV的LTR为启动子,以Luc为报告基因的质粒和以上病毒反式激活因子的表达质粒共转染BL12细胞系,通过瞬时表达分析试验证明了JDV和BIV的LTR和Tat之间亲缘关系很近,能够相互激活;JDV Tat可以反式激活BLVLTR,BLV Tax不能激活JDV LTR;JDV LTR上存在BFV Tas的应答元件;BLV、BFV和BIV的LTR和反式激活因子间不存在相互激活.     

A quantitative assay for measuring of bovine immunodeficiency virus using a luciferase-based indicator cell line

In order to quantitate the bovine immunodeficiency virus (BIV) infection in vitro, a BIV indicator cell line (BIVL) was established by transfecting baby hamster kidney cells with reporter plasmids containing the firefly luciferase gene driven by a BIV long terminal repeat promoter. The BIV activates promoter activity of the LTR to express luciferase upon infection. BIV infection could therefore by quantified by detection of luciferase activity. Compared to standard assays used to detect BIV infection, the BIVL-based assay is 10 times more sensitive than the the CPE-based assay, and has similar sensitivity with the viral capsid protein Western blot assay. BIV indicator cell line could detect BIV infection specifically. Luciferase activity of BIV infected BIVL cells showed a time dependent manner, and 60 h post infection is the optimal time to detect BIV infection. Luciferase activity of BIVL cells correlates with the BIV capsid protein expression. Moreover, a linear relationship was found between MOI and the activated intensity of luciferase expression. In brief, the BIV indicator cell line is an easy, robust and quantitive method for monitoring BIV infection.     

A Quantitative Assay for Measuring of Bovine Immunodeficiency Virus Using a Luciferase-based Indicator Cell Line

In order to quantitate the bovine immunodeficiency virus (BIV) infection in vitro, a BIV indicator cell line (BIVL) was established by transfecting baby hamster kidney cells with reporter plasmids containing the firefly luciferase gene driven by a BIV long terminal repeat promoter. The BIV activates promoter activity of the LTR to express luciferase upon infection. BIV infection could therefore by quantified by detection of luciferase activity. Compared to standard assays used to detect BIV infection, the B...     

牛免疫缺陷病毒反式激活因子功能域的研究

牛免疫缺陷病毒 (Ｂｏｖｉｎｅｉｍｍｕｎｏｄｅｆｉｃｉｅｎｃｙｖｉｒｕｓ,ＢＩＶ )与人免疫缺陷病毒 (Ｈｕｍａｎｉｍ ｍｕｎｏｄｅｆｉｃｉｅｎｃｙｖｉｒｕｓ,ＨＩＶ)同属反转录病毒科慢病毒属[1] 。ＢＩＶ基因组 5′端的长末端重复序列 (ＬＴＲ)起始病毒结构基因和非结构基因的转录[2 ] ,因而许多细胞因子和病毒编码的调节蛋白作用于ＬＴＲ ,以调节ＢＩＶ的基因表达。其中Ｔａｔ蛋白是ＢＩＶ的反式激活因子 ,可大大提高ＬＴＲ的转录水平 ,在ＢＩＶ的基因表达及基因组复制的调节中起重要作用[3 ] 。ＨＩＶ、马传染性贫血病毒 (Ｅｑｕｉ…     

Preparation of BFV Gag antiserum and preliminary study on cellular distribution of BFV

Viruses (e.g. Human immunodeficiency virus, Human simplex virus and Prototype foamy virus) are obligate intracellular parasites and therefore depend on the cellular machinery for cellular trafficking. Bovine foamy virus (BFV) is a member of the Spumaretrovirinae subfamily of Retroviruses, however, details of its cellular trafficking remain unknown. In this study, we cloned the BFV gag gene into prokaryotic expression vector pET28a and purified the denaturalized Gag protein. The protein was used to immunize BALB/c mouse to produce antiserum, which could specifically recognize the BFV Gag protein in BFV-infected cells through western blot assay. Additionally, these results demonstrated that both the optimal and suboptimal cleavage of Gag protein occur in BFV-infected cells. Subsequently, the Gag antiserum was used to investigate subcellular localization of BFV. In immunofluorescence microscopy assays, colocalization microtubules (MTs) and assembling viral particles were clearly observed, which implied that BFV may transport along cellular MTs in host cells. Furthermore, MTs-depolymerizing assay indicated MTs were required for the efficient replication of BFV. In conclusion, our study suggests that BFV has evolved the mechanism to hijack the cellular cytoskeleton for its replication.     

Subcellular localization analysis of bovine foamy virus Borf1 protein

The Borf1 protein is encoded by an immediate-early gene of the bovine foamy virus (BFV) and plays a key role in the viral life cycle. Borf1 is a DNA binding protein which can transactivate both the long terminal repeat (LTR) and the internal promoter (IP) of BFV by specifically binding to the transactivation responsive element (TRE). To analyze the subcellular localization of Borf1 during the BFV life cycle, this gene was cloned into a prokaryotic expression vector and expressed in a soluble form. After the purification and immunization, we raised the mouse anti-Borf1 serum with a high titer based on ELISA results. Western blot analysis showed that the antiserum could specifically recognize the Borf1 protein that was expressed in 293T cells. With this specific serum, we revealed the nuclear and cytoplasmic localization of Borf1 in HeLa cells that was transfected with Borf1. Moreover, the immuno-fluorescence assay also showed that the localization of Borf1 during the infection and transfection of BFV was identical.     

Subcellular Localization Analysis of Bovine Foamy Virus Borfl Protein

The Borfl protein is encoded by an immediate-early gene of the bovine foamy virus （BFV） and plays a key role in the viral life cycle. Borfl is a DNA binding protein which can transactivate both the long terminal repeat （LTR） and the internal promoter （IP） of BFV by specifically binding to the transactivation responsive element （TRE）. To analyze the subcellular localization of Borfl during the BFV life cycle, this gene was cloned into a prokaryotic expression vector and expressed in a soluble form. After the purification and immunization, we raised the mouse anti-Borfl serum with a high titer based on ELISA results. Western blot analysis showed that the antiserum could specifically recognize the Borfl protein that was expressed in 293T cells. With this specific serum, we revealed the nuclear and cytoplasmic localization of Borfl in HeLa cells that was transfected with Borfl. Moreover, the immuno-fluorescence assay also showed that the localization of Borfl during the infection and transfection of BFV was identical.