表达单纯疱疹病毒Ⅱ型糖蛋白D的重组痘苗病毒活疫苗…

我们以前曾报道，表达单纯疱疹病毒Ⅱ型糖蛋白的重组痘苗病毒能保护被免疫小鼠抵抗致死量ＨＳＶ－２病毒的攻击。在此工作基础上，严格按人用疫苗研究要求的实验条件，成功地建立了表达ＨＳＶ－２ｇＤ的重组痘苗病毒活疫苗株，首先将经聚合酶链反应修饰的ＨＳＶ－２ｇＤ基因插入痘苗表达质粒ｐＪＳＢ１１７５，置于痘苗病毒Ｐ７．５Ｋ早／晚期启动子控制下，将同位重组质粒用Ｌｉｐｏｆｅｃｔｉｎ方法转染已受野型ＴＫ＾＋痘苗病毒天     

丙型肝炎病毒结构蛋白在痘苗病毒中的表达

为研究中国丙型肝炎病毒（ＨＣＶ）的抗原性及在细胞内的加工，将丙型肝炎病毒（ＨＣＶ）５’非编码区（ＮＴＲ）和结构基因（Ｃｏｒｅ＋Ｅ１＋Ｅ２／ＮＳ１）插入痘苗病毒表达载体ｐＪＳＡ１１７５中，转染ＴＫ－１４３细胞，经纯化得到丙型肝炎（ＨＣＶ）重组痘苗病毒ｖＪＳＡ１１７５ＣＥ株。Ｓｏｕｔｈｅｒｎｂｌｏｔ杂交表明，ＨＣＶ结构基因存在于痘苗病毒之中。Ｗｅｓｔｅｒｎｂｌｏｔ分析发现，ｖＪＳＡ１１７５ＣＥ表达蛋白带位于９０ｋＤａ，为一多聚蛋白；此蛋白为分泌型，分泌量与细胞裂解物内量大致相同     

应用痘苗病毒载体表达猴轮状病毒VP4抗原基因

把编码猴轮状病毒（Ｒｈｅｓｕｓｒｏｔａｖｉｒｕｓ，ＲＲＶ）Ｖｐ４抗原的第４基因片段插入到痘苗病毒表达载体ｐＪＳＡ１１７５的Ｐ７．５启动子下游，构建成在痘苗病毒Ｐ７．５启动子调控下表达猴轮状病毒Ｖｐ４抗原基因的重组质粒ＰＪＳＡ１１７５－ＶＰ４。应用磷酸钙沉淀技术将ＰＪＳＡ１１７５－ＶＰ４ＤＮＡ转入ＴＫ－１４３细胞，在ＢＵＤＲ和Ｘ－ｇａｌ存在下筛选蓝色蚀斑。经３代以上纯化和病毒增殖，获重组病毒Ｒ－ＶＪＳＡ１１７５－Ｖｐ４。蚀斑滴定其满度达到１５×１０１１ＰＦＵ／Ｌ。经核酸杂交试验证明所获得的重组痘苗病毒带有猴轮状病毒Ｖｐ４抗原基因。用重组病毒感染ＴＫ－１４３细胞（或Ｖｅｒｏ细胞），在感染后４８ｈ，用酶免疫法（ＥＩＡ）检测受染细胞上清液和细胞裂解液中表达的猴轮状病毒Ｖｐ４抗原基因均呈阳性反应。本试验为本研究室轮状病毒基因工程疫苗的一部分，为深入了解轮状病毒基因结构及其功能在方法学上奠定了必要的基础。     

狂犬病毒糖蛋白及核蛋白在非复制型痘苗病毒天坛 …

目的 提高重组痘苗病毒狂犬疫苗的有效性和安全性。方法 利用ＴＫ区表达狂犬病毒糖蛋白（ＲＧ）的重组痘苗病毒作为亲本株，通过两步同源重组，删除痘苗病毒基因组ＣＫ片段间与毒力和宿主范围相关的核酸片段，同时将狂犬病毒核蛋白（ＲＮ）基因插入Ｃ－Ｋ片段之间，获得了含有ＲＧ基因和ＲＮ基因的非复制型重组痘苗病毒ＶＴＫＲＧ△ＣＫＬａｃＺＲＮ。结果 经ＰＣＲ鉴定，ＲＮ基因已插入ＣＫ区；Ｗｅｓｔｅｒｎ ｂｌｏｔ结果显示     

应用痘苗病毒体表达猴轮状病毒VP4抗原基因

把编码猴轮状病毒Ｖｐ４抗原的第４基因片段插入到痘苗病毒表达载体ｐＪＳＡ１１７５的Ｐ７．５启动子下游，构建成在痘苗病毒Ｐ７．５启动子调控下表达猴轮状病毒Ｖｐ４抗原基因的重组质粒ｐＪＳＡ１１７５－Ｖｐ４。应用磷酸钙沉淀技术将ｐＪＳＡ１１７５－Ｖｐ４ＤＮＡ转入ＴＫ－１４３细胞，在ＢＵＤＲ和Ｘ－ｇａｌ 存在下筛选蓝色蚀斑。     

HSV—1 SM44株糖蛋白D基因真核表达载体的构建及其免？…

目的 构建ＨＳＶ－１型ＳＭ４４株糖蛋白Ｄ（ｇＤ）基因的真核表达载体,并用此重组质粒直接免疫小鼠,探讨ＨＳＶ－１ ｇＤ基因作为基因疫苗的可能性。方法 从ＨＳＶ－１基因组中扩增ｇＤ的全编码基因,克隆入载体ｐＵＣ１９中,测序鉴定后转入真核表达载体ｐｃＤＮＡ３．１（＋）。所得重组质粒ｐｃＤ－ＮＡ－ｇＤ以电穿孔法转染ＣＨＯ细胞,并以荧光染色法鉴定表达效果。用ｐｃＤＮＡ－ｇＤ免疫小鼠,ＥＬＩＳＡ法检测基因免疫     

核酶对鸭乙型肝炎病毒感染体内抗病毒作用效果的观察

目的观察核酶在体内抗病毒作用效果。方法选择鸭乙型肝炎（ＤＨＢＶＬＪ－７６）及其鸭动物模型作为检测系统，将针对ＤＨＢＶＰｒｅ－Ｓ７３６位点的核酶（ＲｚＤＳ）插入ｐＪ１２０质粒构建成ｐＪ－ＲｚＤＳ。与痘苗病毒天坛７６１株（ＶＶ）同源重组后获得含ＲｚＤＳ的重组痘苗病毒（Ｖ－ＲｚＤＳ）。用ＤＨＢＶ感染１日龄北京鸭，分别在感染的同时、感染后２４小时和７２小时注射Ｖ－ＲｚＤＳ和ＶＶ，１０天后检测血清中ＤＨＢＶＤＮＡ和ＤＨＢｓＡｇ的含量。结果北京鸭在感染ＤＨＢＶ的同时注射Ｖ－ＲｚＤＳ，其ＤＨＢＶＤＮＡ和ＤＨＢｓＡｇ的含量均低于ＶＶ对照组，两组之间有显著性差异。结论提示ＲｚＤＳ对ＤＨＢＶ基因组复制和表达均有抑制作用，其抑制率分别为４５％和６３％。     

中国狂犬病毒疫苗株（5aG）糖蛋白基因在痘苗病毒中的表达及免疫效果观察

将克隆到的中国狂犬病毒疫苗株（５ａＧ）的糖蛋白基因重组到痘苗病毒ＴＫ区，并在痘苗病毒Ｐ１１启动子的控制下，构建了狂犬－痘苗重组病毒（ＶＶａＧ）。经间接免疫荧光和Ｗｅｓｔｅｒｎ免疫印染证明，重组病毒ＶＶａＧ能良好地表达狂犬病毒糖蛋白，其分子量约为６６００。用ＶＶａＧ免疫小鼠，７ｄ便可诱生较高的狂犬病毒中和抗体，２１ｄ达４１６９，并能１００％保护狂犬病毒本毒株和国际标准攻击毒（ＣＶＳ）的致死量攻击。     

人免疫缺陷病毒1(HIV-1)膜蛋白基因片段在酵母中的克隆表达

目的为获得足够量的膜糖蛋白,以便于对不同ＨＩＶ分离株膜糖蛋白的结构与功能进行进一步的研究。方法从人免疫缺陷病毒１（ＨＩＶ－１）ＨＸＢ２分离株原病毒基因组的重组质粒ｐＨＸＢ２中克隆了两段膜糖蛋白基因（ＥＮＶ）片段。以酵母穿梭诱导表达质粒ｐＹＥＳ２为载体,构建了两个相应的重组表达质粒ｐＹＥＮＶ１和ｐＹＥＮＶ２;进一步利用大肠杆菌β－半乳糖苷酶基因（β－ｌａｃＺ）构建了ＨＩＶ－１膜外糖蛋白ＤＮＡ片段与β－ｌａｃＺ基因的融合表达质粒。将此３种质粒分别转化单细胞真核生物酿酒酵母ＢＪ１９９１,得到的转化子经半乳糖诱导表达后进行菌体全蛋白的ＳＤＳ－ＰＡＧＥ分析。结果克隆的基因片段在酿酒酵母中产生了分子质量为５０×１０３的特异性诱导蛋白;对含此融合表达质粒的酵母转化子半乳糖诱导后表达产物的免疫检测表明,与对照菌株相比,融合表达产物具有和ＨＩＶ－１阳性血清抗体反应的抗原性。结论可通过β－半乳糖苷酶活性的测定直接指示抗原片段的表达;为表达的膜糖蛋白片段的进一步分离纯化打下了一定基础     

蓝舌病毒两外壳蛋白VP2和VP5在昆虫细胞中的表达 …

目的 研究蓝舌病毒（ＢＴＶ）ＶＰ２与ＶＰ５的免疫学特性,为ＢＴＶ基因工程疫苗研究和病毒样颗粒装配打下基础。方法 将ＢＴＶ１０ ＶＰ２和ＶＰ５基因分别插入杆状病毒表达载体ｐＦａｓｔＢａｃ１,转染昆虫细胞获得重组杆状病毒。用ＳＤＳ－ＰＡＧＥ和Ｗｅｓｔｅｒｎ ｂｌｏｔ检测重组杆状病毒对ＶＰ２和ＶＰ５的表达,运用组织培养中和试验和直接血凝试验检测表达产物的生物学活性。     

Construction of recombinant fowlpox viruses as vectors for poultry vaccines

Plasmid vectors have been constructed which allow the construction of infectious fowlpox virus (FPV) recombinants expressing foreign genes. The foreign genes were inserted within the thymidine kinase (TK) gene of FPV contained in these vectors. To facilitate the selection of recombinants the Escherichia coli xanthine guanine phosphoribosyl transferase (Ecogpt) gene was developed as a dominant selectable marker. This marker operates in a wide variety of cell types and obviates the need for TK⁻ cell lines for selection of TK⁻ recombinants when foreign genes have been inserted within the TK gene of FPV. The general approach adopted was to construct plasmid vectors in which the FPV TK was interrupted by the Ecogpt gene under the control of a poxvirus promoter in tandem with a gene of interest under the control of another poxvirus promoter. Selection of viruses expressing the Ecogpt gene simultaneously selects for recombinants carrying both the Ecogpt gene and the gene of interest. Using this approach a series of plasmid vectors was constructed in which the FPV TK gene was interrupted by the Ecogpt gene under the control of the P7.5 vaccinia virus promoter in tandem with the A/PR/8/34 haemagglutinin gene under the control of the PL11 vaccinia virus promoter. A recombinant FPV constructed using these plasmids had the expected genome arrangement, expressed influenza haemagglutinin, and induced haemagglutination-inhibiting antibodies when inoculated into chickens. These techniques should allow the construction of a variety of recombinant FPVs expressing poultry vaccine antigens. Such recombinants should be a very cost-effective means of delivering vaccines to poultry.     

Transactivation by herpes simplex virus proteins ICP4 and ICP0 in vaccinia virus infected cells.

Vaccinia virus recombinants containing the sequences from herpes simplex virus type 1 (HSV-1) encoding the immediate early (IE)(alpha) proteins ICP4 and ICP0, under the control of a mutated vaccinia virus 11K late promoter, were constructed. A cDNA copy of the gene encoding ICPO and an ICP4-encoding genomic segment were each inserted into the vaccinia virus genome at the thymidine kinase (TK) locus by homologous recombination. Steady-state analyses revealed that RNAs homologous to the IE-0 and IE-4 sequences accumulated in cells infected by recombinants with the kinetics of a typical vaccinia late mRNA. Western blot analyses demonstrated that the expression level of both ICPO and ICP4, produced by the recombinant viruses, was comparable to that in HSV-1-infected cells at late times postinfection. Both proteins synthesized in cells infected by the recombinants were located in the nucleus as revealed by immunofluorescence. Although in vitro studies reveal that extracts from vaccinia-virus-infected cells lose the ability to transcribe genes that contain RNA polymerase II promoters (Puckett and Moss (1983), Cell 35, 441-448) both ICPO and ICP4 expressed by the recombinant viruses can transactivate plasmids containing a reporter gene driven by the promoters for the HSV-1 TK and glycoprotein C genes. Nuclear extracts prepared from cells infected with the vaccinia virus vector expressing ICP4 exhibited sequence-specific DNA-binding activity.     

表达HPV18E7E6的重组痘苗病毒构建及免疫效果的初步研究

目的 构建表达HPV18E7E6融合蛋白的重组痘苗病毒,并对E7E6蛋白的免疫原性进行研究.方法 将去除了转化活性的HPV18E6、E7基因融合,插入痘苗病毒重组质粒,通过同源重组构建表达HPV18E7E6的重组痘苗病毒,观察其免疫效果.结果 构建了表达E7E6融合蛋白的重组痘苗病毒,PCR鉴定及测序表明融合基因序列与设计相符,正确插入到痘苗病毒TK区域;Western-Blot检测表明该重组病毒能表达HPV18E7E6融合蛋白.免疫后的小鼠可产生E6、E7特异性抗体,但ELISPOT没检测到E7肽库刺激小鼠脾细胞产生分泌IFN-丫的阳性反应.结论 构建了一株表达HPV18E7E6融合蛋白的重组痘苗病毒,可以有效诱发小鼠产生针对E6、E7的体液免疫,但不能诱发产生相应的细胞免疫,为进一步研究不同动物模型中HPV18E6E7的细胞免疫特点提供了实验基础.     

Construction of recombinant swinepox viruses and expression of the classical swine fever virus E2 protein

To explore the swinepox virus (SPV) as a potential live vector for immunization, a vector was developed for the construction of a recombinant SPV carrying foreign genes. In this system, a foreign gene placed under the strong vaccinia virus promoter P(11) can be inserted into the viral thymidine kinase (TK) gene, and the recombinant virus can be isolated in a non-selective medium by the co-expression of E. coli lacZ gene. Compared with the wild type virus, the TK(-)recombinant SPV showed a modest level of attenuation in porcine cells while more attenuation was observed in monkey or human cells. Using this system, a recombinant virus expressing the E2 glycoprotein of classical swine fever virus (CSFV) was produced. Engineered with the gX signal sequence of the pseudorabies virus, and transmembrane domain of E2, the E2 protein was expressed as a dimeric form in the cytoplasm of the infected cells.     

人粒细胞巨噬细胞集落刺激因子在重组痘苗病毒中的 …

目的 观察人ＧＭ－ＣＳＦ（粒细胞－巨噬细胞集落刺激因子）对重组痘苗病毒免疫效果的影响。方法 大鼠体内观察。结果 从核酸和蛋白水平均证实重组痘苗病毒ＲＶＪＳＢ１１７５Ｄ／ＧＭ－ＣＳＦ可同时表达ＧＭ－ＣＳＦ及ＨＳＶ－１ｇＤ（单纯疱疹病毒ｇＤ糖蛋白），但ＲＶＪＳＢ１１７５Ｄ／ＧＭ－ＣＳＦ免疫大鼠产生的抗－ＨＳＶ１ｇＤ特异性抗体水平与ＲＶＪＳＢ１１７５Ｄ组相比无显著性差异。结论 人ＧＭ－ＣＳＦ在大鼠体内对     

Simultaneous expression of the Lassa virus N and GPC genes from a single recombinant vaccinia virus

A new transfer vector was constructed that directs the insertion of two heterologous genes into the vaccinia virus thymidine kinase (TK) gene during a single recombination event. This vector, pDAVAC2, contains bidirectional vaccinia P7.5 early/late promoter elements and two unique cloning sites. cDNA clones containing the complete coding sequences for the Lassa virus (Josiah strain) nucleoprotein (N) and glycoprotein (GPC) genes were inserted into the vaccinia TK gene using this transfer vector. The recombinant virus, V-LSGN-II, expressed proteins in cell culture that appeared to be authentic with respect to electrophoretic mobility, glycosylation, and post-translational cleavage. Indirect immunofluorescence (IFA) of recombinant virus-infected cells demonstrated both the bright granular and diffuse patterns of staining characteristic of the Lassa nucleoprotein and glycoprotein, respectively. Electron-dense inclusion bodies typical of arenavirus-infected cells were observed by electron microscopy in V-LSN and V-LSGN-II-infected cells, but not in V-LSGPC-infected cells. Mice inoculated with V-LSGN-II by intraperitoneal injection developed serum antibodies that reacted with authentic Lassa proteins in immunofluorescence and radioimmune precipitation assays. This recombinant virus represents an additional candidate for a Lassa fever vaccine and demonstrates the feasibility of expressing any two genes of interest in a single recombinant vaccinia virus through the use of the transfer vector pDAVAC2.     

共表达HIV-1 gag-gp120与白细胞介素6重组鸡痘病毒的筛选

目的构建共表达中国株HIV1gaggp120与白细胞介素6(IL6)的重组鸡痘病毒(FPV)。方法分别将HIV1gaggp120基因和IL6基因插入到FPV表达质粒pUTAL复合启动子和单一启动子下游,构建重组FPV表达质粒pUTAGEIL6。利用脂质体法将重组质粒和FPV282E4株共转染鸡胚成纤维细胞,经BUdR加压筛选,重组病毒分别用SDSPAGE和WesternBolt进行鉴定,观察病毒样粒子的形成和重组病毒在哺乳动物细胞中的表达,并分析其免疫原性。结果阳性重组病毒基因组点膜处有显色斑点,WesternBolt结果显示重组病毒表达了gaggp120嵌合蛋白和IL6,在病毒感染细胞中有反转录病毒样粒子形成,且重组病毒可在哺乳动物细胞中表达目的蛋白。小鼠免疫指标检测表明该重组病毒具有很好的免疫原性。结论成功构建了共表达中国株HIV1gaggp120与IL6的重组FPV,为HIV-1基因工程活载体疫苗和巨分子颗粒化疫苗的制备奠定了基础。     

Construction of a pigeonpox virus recombinant: expression of the Newcastle disease virus (NDV) fusion glycoprotein and protection of chickens against NDV challenge

Summary A pigeonpox transfer plasmid was constructed by cloning a 2.5 kb DNA fragment containing the viral thymidine kinase (TK) gene in the psp65 plasmid. The vaccinia virus P11K promoter followed by the NDV fusion (F) gene was inserted in the TK gene. The F gene was transferred to the viral genome by homologous recombination in pigeonpox virus infected CEF cells, transfected with the recombinant plasmid. Recombinant viruses were selected with BUdR and screened for their ability to induce fusion between adjacent cells. Because of the unexpected growth advantage of the TK+ WT over the TK– recombinants, viral purification was needed to obtain stable recombinants expressing a glycosylated and cleaved F protein. Vaccination of chickens by the follicular method induced high anti-F antibody titers and good protection against challenge with the virulent Italian NDV strain. Half of the oculonasal vaccinated chickens showed anti F antibodies and also half of them were protected. Although protection seems to be correlated with antibody titers, no neutralizing antibodies were found.