禽痘病毒感染对禽流感重组禽痘病毒疫苗免疫效力的影响

表达禽流感病毒 (AIV)HA和NA基因的重组禽痘病毒rFPV_HA_NA能够诱导鸡体产生 10 0 %抵抗高致病性禽流感病毒 (HPAIV)H5N1的攻击。而当鸡群已进行禽痘疫苗免疫或者感染了禽痘病毒的情况下 ,此重组疫苗的免疫效力如何 ?首先用禽痘病毒S_FPV_0 17人工感染SPF试验鸡 ,既而在感染后的不同间隔时间接种重组疫苗 ,免疫后检测鸡群的HI抗体水平 ,同时用 10 0LD50 的HPAIVH5N1进行攻击。结果重组疫苗免疫与禽痘病毒人工感染时间间隔在 4周 (或以上 )时 ,预先感染禽痘病毒对重组疫苗的免疫效力不构成影响 ,对禽流感的保护力为 10 0 % ,而间隔时间在 1、2、3周时 ,重组疫苗的免疫保护效力则受到不同程度的影响。     

Structural proteins of bovine parainfluenza-3 virus

Six structural proteins of bovine parainfluenza-3 virus (PI-3V) labeled with [35S]-methionine could be resolved by polyacrylamide gel electrophoresis (PAGE). Five structural proteins of this virus had been previously reported. The 6 proteins found in this study were: L, a 180,000 (180 kD) molecular weight (MW) large protein; P, 83 kD phosphoprotein; HN, 69 kD hemagglutinin-neuraminidase glycoprotein; NP, 66 kD nucleocapsid protein; F, 55 kD fusion glycoprotein; and M, 38 kD matrix protein. Selective labeling with [2-3H]-mannose revealed only HN and F glycoprotein bands. A cellular actin protein (43 kD), associated with many enveloped viruses, was also found as a seventh protein in bovine PI-3V.     

Isolation of surface tubules of fowlpox virus

Surface tubules of fowlpox virus were isolated using chemical and physical methods. Suspensions of lipid cytoplasmic inclusion bodies were obtained by treating infected chorioallantoic membranes with 1% trypsin. Inclusions were treated with ultrasonic sound, detergents, and enzymes and were examined by electron microscopy. Although lipase treatment altered the morphology of lipid inclusions, no viral surface tubules were recovered. Treatment with the detergent Nonidet-P40 followed by 2-mercaptoethanol disrupted virions without allowing surface tubules to be recovered. Disruption of lipid inclusions by ultrasonic sound or manual grinding of chorioallantoic membranes produced free virions but only small numbers of tubules. These results indicate that surface tubules can be recovered, but that the lipid nature of cytoplasmic inclusions interferes with procedures commonly used in tubule purification.     

禽痘病毒载体疫苗研究进展

禽痘病毒和其它痘病毒一样,基因组的高保守区的非复制域可以整合外源DNA,已成为普遍的表达载体,主要应用于痘病毒分子生物学领域、体外生产和蛋白质功能化研究以及作为活的疫苗或工具用于疫苗研究.禽痘病毒载体疫苗不仅能预防禽痘的发生,而且通过插入多个其它病原的保护性抗原基因以诱导产生抗外来抗原的抗体和细胞毒性T细胞反应,提高对相应病原的免疫抵抗力.由于重组病毒所表达的外源基因在机体内随载体病毒的复制而表达,与灭活疫苗相比,它容易生产,免疫剂量小,接种方法简便,接种一次就能获得长期的免疫效果,大大降低了生产成本.     

Structural proteins of bovine viral diarrhea virus.

A procedure for the purification of radioactively labeled bovine viral diarrhea virus was critically evaluated. Purification of virus from artificial mixtures of unlabeled infected and labeled noninfected cells indicated that the extent of purification was approximately 100-fold with respect to host proteins. Residual host proteins were found to contaminate the viral preparation even after extensive purification by differential and isopycnic zonal centrifugation. Co-electrophoresis of 3H-labeled virus with 14C-labeled host cell material in neutral sodium dodecyl sulfate-7.5% polyacrylamide gels provided a means to distinguish viral specific proteins from host cell protein contaminants. Four major electrophoretic components were identified as being of viral origin; molecular weights of the components were estimated from their migration rates relative to protein markers of known molecular weight. Two viral components (VC), VC 1 and VC 3, migrated heterogeneously and had molecular weights of 93,000 to 110,000 and 50,000 to 59,000 daltons, respectively. Molecular weights of VC 2 and VC 4 were 70,000 and 25,000 daltons, respectively.     

Expression of avian influenza virus hemagglutinin by recombinant fowlpox virus

A vaccine strain of fowlpox virus (FPV) was genetically engineered to produce avian influenza virus hemagglutinin (HA). This was accomplished by inserting a cDNA copy of the avian influenza virus HA gene, which was regulated by a vaccinia virus promoter, into the FPV thymidine kinase (TK) gene. Two types of recombinant viruses, differing only in the orientation of the HA gene relative to an adjacent foreign gene (lacZ), were created. Following preliminary identification of FPV recombinants based on the generation of beta-galactosidase (lacZ gene product), correct insertion of the HA gene into the genomes of these viruses was verified by hybridization studies. Susceptible chickens vaccinated with these FPV recombinants produced specific hemagglutination-inhibiting antibodies against the HA antigen. In view of this immune response, these viruses may serve as vaccines against avian influenza virus. In this regard, they appeared to be less virulent than the parental virus.     

表达传染性喉气管炎病毒gB基因重组鸡痘病毒疫苗免疫持续期试验

将200003批疫苗免疫4周龄SPF鸡,免疫后的7、14、21、30、60、90、120、150、180和225 d分别采血,分离血清,采用ELISA方法检测血清抗FPV抗体,结果表明重组疫苗免疫后14 d,免疫鸡血清抗体已经全部阳转,免疫后的21 d血清抗FPV的抗体出现峰值,此后便开始下降,到免疫后的6个月抗体水平已经接近阴性对照的水平.用ILTV WG株和FPV 102株强毒进行的攻毒保护试验与血清检测的结果基本一致,在免疫后的5个月内可以使免疫鸡获得100%(10/10)保护,免疫后的6个月对ILT和FP的免疫保护分别为1/7和2/10,此时需要对鸡群实施二次免疫.其他5批疫苗(200001、200002、200101、200102和200103)免疫SPF鸡后5个月用ILTV WG株和FPV 102株攻击也获得了完全保护.     

以GPT和GFP为双重筛选标记的禽痘病毒转移载体的构建及鉴定

为研制和开发以禽痘病毒为载体的重组病毒疫苗,本研究构建了禽痘病毒通用转移载体pSY681-gfp-gpt,该载体含有gfp和gpt2种报告基因及背对的痘苗病毒晚期启动子P11和早期启动子P7.5,P11启动gfp和gpt两个基因,P7.5用于启动外源基因,在早期启动子P7.5下游引入NotⅡ和AftⅡ两个酶切位点.用于外源基因的插入.为检测禽痘病毒转移载体pSY681-gfp-gpt的有效性,将H9亚型禽流感病毒A/Chicken/Shanghai/10/01(H9N2)的HA基因插入到该载体中构建转移载体pSY681-gfp-gpt-HA9,将转移载体转染已感染禽痘病毒S-FPV-017的鸡胚成纤维细胞,利用gfp和gpt同时进行双重筛选、数轮蚀斑纯化后获得了重组病毒rFPV-gpt-gfp-HA9,通过PCR、western blot鉴定,结果证明,获得了能稳定表达H9亚型禽流感病毒HA蛋白的重组禽痘病毒rFPV-gpt-gfp-HA9,为今后重组禽痘病毒活载体疫苗的研制奠定了基础.     

Regulation of foreign gene in fowlpox virus by a vaccinia virus promoter

A vaccinia virus promoter was evaluated for regulation of a foreign gene in fowlpox virus by a transient expression assay. Fowlpox virus-infected quail cells, transfected with plasmid DNA containing chloramphenicol acetyltransferase (CAT) gene ligated to a vaccinia virus promoter, expressed CAT activity. No CAT activity was detected either in uninfected cells or fowlpox virus-infected cells. These results indicated that a heterologous vaccinia virus promoter can regulate expression of a foreign gene in fowlpox virus.     

表达新城疫病毒融合蛋白基因禽痘病毒重组体的构建

通过RT-PCR扩增新城疫病毒F基因,利用禽痘病毒复合启动子、SV40 PolyA终止信号序列构建F基因表达盒。将F基因表达盒与loxp-GFP-loxP序列串联插入禽痘病毒重组臂,构建了禽痘病毒转移质粒载体。在脂质体介导下转染CEF,获得了带有绿色荧光信号的重组病毒rFPVFGFP。通过二次转染,利用Cre-loxP位点特异性重组将重组病毒基因组的GFP自动去除,结果获得了只含新城疫病毒F基因表达盒的重组禽痘病毒rFPVF。试验结果表明,rFPVF复制稳定,表达的F蛋白具有免疫原性,能够刺激鸡只产生抗新城疫病毒的中和抗体。     

Vaccination of chickens with a recombinant fowlpox virus containing the hemagglutinin-neuraminidase gene of Newcastle disease virus under the control of the fowlpox virus thymidine kinase promoter.

When chickens were vaccinated with a recombinant fowlpox virus (FPV) containing the Newcastle disease virus (NDV) hemagglutinin-neuraminidase (HN) cDNA under the control of the thymidine kinase (TK) promoter and inserted into the FPV TK gene, the FPV antibody response to the recombinant virus was similar to the response to vaccination with standard FPV, and the recombinant virus protected chickens against challenge with virulent FPV. While the presence of the NDV HN cDNA was demonstrated in the recombinant virus, which was stable on serial passage, expression of HN was not detected by hemagglutination, Western blot analysis or immunoprecipitation of infected cell lysate. Chickens vaccinated with the recombinant virus failed to mount an NDV hemagglutination-inhibition antibody response, and they did not resist challenge with velogenic NDV. It was concluded that the TK promoter was too weak to drive the HN gene, but that the insertion into the FPV TK gene did not reduce the immunogenicity of the virus.     

表达传染性支气管炎病毒S1基因重组鸡痘病毒的构建

将鸡传染性支气管炎病毒S1基因插入到鸡痘病毒转移载体pSY681中，获得重组转移载体pSY681。将pSY681-IBVS1转染已感染亲本鸡痘病毒S-FPV-017株的鸡胚成纤维细胞，使其在鸡胚成纤维细胞内与鸡痘病毒基因组发生同源重组，产生表达鸡IBVS1蛋白的重组鸡痘病毒rFPV-IBVS1。在含有X-gal的营养琼脂培养基上进行蓝斑筛选且进一步纯化14代。S1基因的PCR检测表明，获得的含传染性支气管炎病毒S1基因的重组鸡痘病毒能够稳定遗传，间接免疫荧光和Western blot等试验证实该重组病毒在CEF内真实地表达了分子量约为90Ku的具有免疫学活性的IBV S1糖蛋白。     

利用Cre-loxP自动去除禽痘病毒重组体的报告基因

在含痘病毒早晚期启动子的绿色荧光蛋白(GFP)基因表达盒侧翼各引入1个loxP序列。以禽痘病毒282E4株作为候选载体,通过同源重组将其插入到病毒基因组的FPV030区域,获得了表达GFP的重组禽痘病毒。然后在Cre酶介导下,利用loxP位点特异性重组剪除了重组病毒基因组中的GFP报告基因。结果表明,以GFP作为筛选标记使重组病毒的构建更为简便,同时利用Cre-loxP系统可以轻松地去除报告基因。这种技术有利于其它抗原性基因重组禽痘病毒的构建。     

表达NDV HN基因的重组鸡痘病毒的部分生物学特性研究

为了评价转基因对鸡痘病毒(FPV)生物学特性的影响,通过电镜观察表达新城疫病毒(NDV)血凝素-神经氨酸酶蛋白(HN)基因重组鸡痘病毒(rFPV-12LSHN)感染的鸡胚成纤维细胞(CEF).结果表明:在FPV中插入NDV HN基因后,不改变rFPV的形态、病毒成熟过程;rFPV-12LSHN与FPV在CEF上的产量无...     

应用间接ELISA检测鸡痘病毒抗体方法的建立

应用鸡胚成纤维细胞(CEF)扩增鸡痘病毒(Fowlpox virus,FPV)并提纯后作为抗原建立了具有较高特异性和灵敏性的间接ELISA方法.通过方阵滴定法来确定抗原最佳包被浓度为2.7μg/孔,待检血清最佳稀释倍数为1:100,其阳性临界值为OD≥0.113.将400份FPV免疫实验鸡血清用本方法进行检测,其阳性检出率为81.25%(325/400).此外,将该方法与琼脂扩散试验进行比较检测血清样品,结果显示本方法的灵敏度比琼脂扩散试验灵敏400～800倍,而且还有特异性强,操作简便、快速等优点.     

Structural proteins of equine infectious anemia virus and their antigenic activity

Using purified equine infectious anemia (EIA) virus labeled with 3H-glucosamine or 14C-protein hydrolysate, structural proteins were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. As a result, 2 glycoproteins and 10 proteins with molecular weights (mol wt) ranging from 12,000 to 115,000 daltons were demonstrated. Of 12 structural proteins, 3 proteins, namely a glycoprotein with mol wt of 76,000 (gp76) and 2 proteins with mol wt of 25,000 (p25) and 12,000 (p12), respectively, had distinct antigenic activity from one another in immunodiffusion. Development of antibodies against gp76 and p25 was compared in infected horses. The antibody to gp76 appeared earlier and stronger than to p25 in horses infected with the homologous virus strain. The fraction with glycoproteins was found to have hemagglutinating activity which was inhibited by the serum sample from horses infected with equine infectious anemia virus.