Construction of Recombinant Fowlpox Virus(rFpv) Expressing HIV-1 Gag-pol Protein

The induction of human immunodeficiency virus（HIV）-specific T-cell response is generally considered as critical to the development of effective immunity to HIV type 1 （ HIV-1 ）. Recombinant Avipoxvirus vectors are used widely for vaccination against HIV-1, where the induction of a cytotoxic CD8 ＋ T-cell（CTL） response seems to be an important component of protective immunity. A recombinant fowlpox virus（rFPV/Gag-pol） expressing the Gag-pol protein of HIV was constructed and characterized. The specific expression protein in CEF cells infected by recombinant fowlpox and the specific antibody in the sera of mice immunized with rFPV were analyzed via Western-blot.

Immune Efficacy of a Recombinant Fowlpox Virus Co-Expressing HA and NA Genes of Avian Influenza Virus in SPF Chickens

A recombinant fowlpox virus co-expressing Haemagglutinin (HA) and Neuraminidase (NA)named as rFPV-HA-NA was produced by HA and NA gene of A/Goose/Guangdong/3/96(H5N1)isolate of avian influenza virus recombined into the genome of fowlpox virus. In thisstudy, to evaluate its ability of protecting chickens against challenge with a lethaldose of highly pathogenic isolates of avian influenza virus, eight-week-old specific-pathogenic-free (SPF) chickens were vaccinated with recombinant virus or the wildtypefowlpox virus by wing-web puncture. After challenge 4 weeks with 10 LD50 highly pathogenicavian influenza virus H5N1 and H7N1 isolate, all chickens vaccinated with recombinantvirus were protected, while the chickens vaccinated with the wildtype fowlpox virus orunvaccinated controls experienced 100% mortality respectively following challenge. Thiscomplete protection was accompanied by the high levels of specific antibody response tothe respective components of the recombinant virus.

CONSECUTIVE IMMUNIZATION WITH RECOMBINANT FOWLPOX VIRUS AND PLASMID DNA FOR ENHANCING CELLULAR AND HUMORAL IMMUNITY

Objective: To investigate the influence of consecutive immunization on cellular and humoral immunity in mice. Methods: We evaluated a consecutive immunization strategy of priming with recombinant fowlpox virus vUTALG and boosting with plasmid DNA pcDNAG encoding HIV-1 capsid protein Gag. Results: In immunized mice, the number of CD 4 + T cells from splenic lymphocytes increased significantly and the proliferation response of splenocytes to ConA and LPS elevated markedly and HIV-1-specific antibody response could be induced. Conclusion: Consecutive immunization could increase cellular and humoral immunity responses in mice.

Adaptability of Fowlpox Virus in Chicken Embryo Passage Cells

[Objective] To observe whether fowlpox virus （FPV） can proliferate in chicken embryo passage fibroblasts or not and then try to use chicken embryo passage fibroblasts to replace primary chicken embryo cells for FPV culture. [Method] Primary chicken embryo fibroblasts were prepared and subcultured. After FPV were inoculated on the 20th passage fibroblasts, cytopathy was observed. Then, the FPV culture was identified and determined quantificationally. [Result] Specific cytopathy appeared in the FPV-inoculated chicken embryo passage fibroblasts. The titer of the yielded FPV culture reached the standard for production of fowl pox vaccine. Further analysis reveals that the chorioallantoic membrane lesions were caused by FPV. [ Conclusion] FPV can reproduce in chicken embryo passage fibroblasts, and the Uter of FPV cell culture can meet the pro- duction requirements of fowl pox vaccine.

Construction and characterization of a recombinant fowlpox virus containing HIV-1 multi-epitope-p24 chimeric gene in mice

The epidemic of HIV/AIDS is sweeping across the world. It is of great importance to figure out new ways to curb this disease. Epitope-based vaccine is one of these solutions. In this study, a chimeric gene was obtained by combination of a designed HIV-1 multi-epitope gene (MEG) and HIV-1 p24 gene. A re- combinant plasmid pUTA2-MEGp24 was then constructed by inserting MEGp24 gene into the down- stream of the promoter (ATI-P7.5×20) of fowlpox virus (FPV) transfer vector pUTA2. The recombinant plasmid and wild-type FPV 282E4 strain were then co-transfected into CEF cells and homologous re- combination occurred. A recombinant virus expressing HIV-1 protein MEGp24 was screened by ge- nome PCR and Western blot assay. Large scale preparation and purification of the recombinant fowl- pox virus (rFPV) were then carried out. BALB/c mice were immunized intramuscularly with the rFPV for three times on day 0, 14 and 42. Mice were executed and sampled one week after the third inoculation. Anti-HIV-1 antibody in serum and Th1 cytokines in the supernatant of cultured spleen cells were as- sayed by ELISA. The count of T lymphocyte subsets and the CTL activity of spleen lymphocytes were analyzed by flow cytometry and lactate dehydrogenase (LDH) release assay, respectively. The results showed that HIV-1 specific antibody in serum and increased T lymphocyte subsets (CD4+ T, CD8+ T) were detected in the immunization group. CTL target-killing activity and higher secretion of Th1 cyto- kines (IFN-γ and IL-2) of spleen lymphocytes stimulated by H-2d-restricted CTL peptide were observed in immunized mice. We concluded that the rFPV may induce HIV-1 specific immunity especially cellular immunity in mice.

牛对表达口蹄疫病毒复合多表位基因的重组鸡痘病毒以及DNA疫苗联合免疫的免疫应答

将构建的共表达口蹄疫病毒(foot-and-mouth disease virus,FMDV)复合多表位基因和猪白细胞介素18基因的重组鸡痘病毒活载体疫苗vUTA2-OAT以及DNA疫苗pVRI-OAT,分别以vUTA2-OAT/vVTA2-OAT(首免/加强免疫)、pVRI-OAT/vUTA2-OAT(首免/加强免疫)和vUTA2-OAT/pVRI-OAT(首免/加强免疫)等3种方式接种牛,然后通过间接ELISA、中和试验和T淋巴细胞增殖试验评价其诱导的特异性体液和细胞免疫水平。结果表明,这3种方式均能诱导牛产生特异性的体液免疫及细胞免疫应答,其中pVRI-OAT/vUTA2-OAT联合免疫方式的免疫效果最佳,诱导的中和抗体达1∶64,已接近于常规灭活疫苗免疫方式,而且其可以诱导比灭活疫苗免疫方式高得多的细胞免疫水平(P<0.01)。上述试验结果为进一步进行免疫攻毒试验,并最终筛选出最佳疫苗和免疫程序奠定了基础。

猪2型圆环病毒与O型口蹄疫病毒二联重组鸡痘病毒的构建和筛选

以pUTA2LacZ为真核表达载体,以中国流行株O型口蹄疫病毒(FMDV)NY00株结构蛋白前体P1基因、猪2型圆环病毒内蒙株的衣壳蛋白和复制蛋白基因为目的基因,构建了2个重组质粒作为中间转移质粒,标记为pUTALP1-ORF2和pUTALP1-ORF2ORF1。将这2个重组转移质粒分别酶切鉴定后,与鸡痘病毒野毒(FPV)282E4株共转染鸡胚成纤维细胞。结果显示,重组核酸质粒构建正确,并能进行表达。经5-溴-2-脱氧尿苷(BrdU)加压筛选,挑取单个蚀斑,3次纯化,获得2株重组毒vpUTALP1-ORF2ORF1和vpUTALP1-ORF2。结果表明,这2株重组鸡痘毒在电镜下可形成完整的病毒粒子。

3株表达H5亚型AIV HA基因的重组鸡痘病毒的免疫效力比较

作者旨在探讨鸡痘病毒ORF073或ORF214基因缺失后,在母源抗体存在情况下对重组病毒免疫效力的影响。将构建好的在ORF073或ORF214基因插入H5亚型AIV HA基因的重组鸡痘病毒(rFPVLP-△73LRH5A、rFPVLP-△214LRH5A)及单表达H5亚型AIV HA基因的重组鸡痘病毒(rFPVLP-12LSH5A)分别免疫SPF鸡和商品鸡,检测重组疫苗诱导的免疫效力。结果:3种重组鸡痘病毒在SPF鸡产生较高的HI抗体效价及100%的免疫保护;在HI母源抗体效价为2.45的商品鸡体内基因缺失株重组病毒比rFPVLP-12LSH5A易于清除,抗体上升缓慢而且免疫28 d后HI抗体效价较低,免疫保护率低,分别为16.7%和23.3%;在母源HI抗体效价为0的商品鸡体内基因缺失株重组病毒免疫后产生的抗体效价高,免疫28 d后分别达到3.50和3.17。结果表明在商品鸡体内母源抗体影响下,缺失ORF073或ORF214基因的重组鸡痘病毒的免疫效力降低。

表达口蹄疫病毒复合多表位基因的重组鸡痘病毒以及DNA疫苗在豚鼠中的免疫原性研究

目的评价本课题组构建的共表达FMDV复合多表位基因以及猪白细胞介素18基因的非复制型重组鸡痘病毒活载体疫苗vUTA2-OAT以及DNA疫苗pVRI-OAT诱导FMDV模型动物豚鼠产生特异性体液免疫和细胞免疫的能力。方法将上述2种重组疫苗分别单独或联合接种豚鼠,然后测定FMDV特异性结合抗体、中和抗体和T淋巴细胞增殖反应,并用250ID50的FMDV进行攻击,观察其保护效果。结果这2种重组疫苗均能诱导豚鼠产生特异性的体液免疫及细胞免疫应答。其中以pVRI-OAT/vUTA2-OAT的联合免疫方式的效果最好,其诱导的抗体水平接近于常规灭活疫苗,而细胞免疫水平则比后者高得多。攻击保护结果显示3个重组疫苗组均有一定保护效果,完全保护率和部分保护率分别为1/4和2/4。而PBS对照组发病率为4/4。结论证实了这2种重组疫苗在豚鼠体内具有良好的免疫原性。上述研究结果为FMDV基因工程疫苗的研究奠定了基础。

鸡3种主要DNA病毒多重感染复合PCR检测方法的建立

依据Gen Bank中注册的鸡马立克氏病病毒(MDV)、鸡传染性喉气管炎病毒(ILTV)、鸡痘病毒(FPV)基因组核苷酸序列中的保守序列设计引物,3种病毒各设计3对引物,共计9对引物,经生物学软件筛选后,得到3对相互匹配较佳的引物。3对匹配引物经单一PCR验证后,优化复合PCR反应条件,确定最佳的退火温度、引物浓度和Taq DNA聚合酶浓度;经特异性、敏感性试验及简化PCR试验,建立简易复合PCR检测方法。复合PCR扩增出的3条带大小与预期一致,即228 bp(MDV)、400 bp(ILTV)、499 bp(FPV);建立的复合PCR方法能同时检测出100 fg MDV、ILTV、FPV的DNA。同时依据PCR技术原理,将经典的三温热循环改进为二温热循环试验,即将退火和延伸合并为一步(62℃),缩短了反应时间。建立的3种病毒的复合PCR检测方法具有较高的特异性和敏感性,可以用于临床病料的快速诊断。

口蹄疫三价重组鸡痘病毒疫苗免疫原性研究

目的对本室已经筛选到的共表达O型、A型和Asia1型FMDV复合多表位免疫原基因OAAT与猪IL-18基因的重组鸡痘病毒vUTA-IL18-OAAT的免疫原性进行研究。方法分别用重组病毒毒vUTA-IL18-OAAT、FPV疫苗株和PBS溶液进行小鼠免免疫,每间隔14d加强免疫1次,第3次免疫后10d杀鼠取血清和脾淋巴细胞检测抗体、T淋巴细胞亚群的数量及CTL活性。结果小鼠免疫试验结果表明,与阴性对照组相比,vUTA-IL18-OAAT免疫组的T细胞亚类数量、CTL杀伤活性,抗O型、A型和Asia1型FMDV的特异性抗体水平差异显著。结论vUTA-IL18-OAAT能有效激发机体的细胞和体液免疫反应。

猪繁殖与呼吸综合征病毒三种不同基因活载体疫苗的免疫性研究

用3株构建好的分别表达猪繁殖与呼吸综合症病毒(Porci ne reproduct i ve andr espi r at or y syndr ome vi r us,PRRSV)GP5蛋白,M蛋白和GP5-M融合蛋白的重组鸡痘病毒接种BALB/c小鼠进行免疫学实验,对其诱导小鼠产生体液免疫和细胞免疫反应的潜力进行了评价。结果表明,表达GP5-M融合蛋白的重组鸡痘病毒相对于其他各组能够刺激免疫鼠产生高水平的特异性中和抗体和ELI SA抗体;显著促进IFN-γ的分泌和特异性T淋巴细胞增殖,。提示表达GP5-M融合蛋白的重组鸡痘病毒可显著增强小鼠的体液免疫和细胞免疫,这为防治PRRSV感染的新型疫苗研究提供了新的思路。

猪圆环病毒与口蹄疫病毒二联重组鸡痘病毒的鉴定和BALB/c小鼠的免疫试验

以鸡痘病毒(FPV282E4)为活载体,用猪2型圆环病毒内蒙株的衣壳蛋白、与复制相关蛋白基因及O型口蹄疫结构蛋白基因作为目的基因,经同源重组的方法获得2个重组鸡痘毒,分别命名为:vUTALP1-ORF2-ORF1、vUTALP1-ORF2。在复制、转录和翻译水平对这2个重组毒进行鉴定,结果表明这2个重组毒均能表达目的蛋白。将它们免疫6～8周龄BALB/c小鼠,每隔19d免疫1次,共3次;每10d尾跟采血1次,三免后10d杀鼠取脾。用ELISA方法检测小鼠血清抗体效价,流式细胞仪检测脾T淋巴细胞亚类CD4+、CD8+数量。结果发现2个重组毒试验免疫组均是从最后一次采集的小鼠血清能获得最高的抗体效价,与对照组FPV相比都能产生一定的体液免疫反应,且以vUTALP1-ORF2-ORF1重组毒免疫小鼠产生的血清抗体效价最高;脾T淋巴细胞亚类数量测定发现,免疫试验组的CD4+与CD8+的T细胞亚类总数显著高于对照组(P<0.05),并以vUTALP1-ORF2-ORF1数值较高。结果表明,这2个重组鸡痘毒既能较好的刺激细胞免疫又能产生一定的体液免疫,将作为候选活载体重组鸡痘毒进行本体动物免疫试验研究。

整合禽网状内皮组织增殖病病毒基因的鸡痘病毒野毒株致病性研究

以分离保存的整合禽网状内皮组织增殖病病毒(REV)基因的鸡痘病毒(FPV)野毒株接种CEF细胞,间接免疫荧光试验检测REV,结果未检测到游离REV病毒粒子;以该毒株人工感染7日龄SPF雏鸡,同时设阴性对照,常规免疫新城疫弱毒苗(ND)。接毒后每周采血动态检测NDV抗体、REV抗体、REV病毒血症;同时对试验鸡免疫器官指数、组织学变化动态观察,并对免疫器官的细胞凋亡动态检测。结果表明,整合REV基因的FPV感染后2周可引起鸡REV病毒血症,并产生REV抗体;导致中枢免疫器官发育分化不良,尤其对胸腺的影响最为明显,攻毒2周后,试验组与对照组相比,胸腺指数明显下降(P<0.05);免疫器官主要表现实质细胞数量少,正常结构发育不良,间质结缔组织增生而发生纤维化;细胞凋亡检测证实免疫器官的淋巴细胞和巨噬细胞均有明显的凋亡现象,细胞凋亡是引起免疫器官萎缩的主要原因。对新城疫疫苗免疫反应呈显著的抑制作用,攻毒3周后,试验组血清新城疫病毒抗体滴度显著低于对照组(P<0.05),其抗体滴度峰值低,维持时间短,下降速度快。本试验证实FPV整合REV前病毒基因组会明显改变FPV的致病性,表现某些REV的致病特征,使感染鸡REV抗体转为阳性并出现病毒血症,进一步证实REV可以通过基因组整合于FPV而进行传播的推测。

缺失ORF73或ORF214基因对重组鸡痘病毒免疫应答的影响

【目的】旨在研究鸡痘病毒ORF73和ORF214编码蛋白是否具有IL-18结合蛋白的功能,以及ORF73或ORF214基因缺失后对重组病毒诱导免疫应答的影响。【方法】以缺失ORF73或ORF214基因并表达H5亚型AIVHA基因的重组鸡痘病毒(rFPVLP-△73LRH5A、rFPVLP-△214LRH5A)作为研究对象,以未缺失ORF73或ORF214基因而表达H5亚型AIVHA基因的重组鸡痘病毒(rFPVLP-12LSH5A)作为对照,检测重组病毒体外诱导SPF鸡脾细胞和外周血淋巴细胞产生IFN情况,同时检测重组病毒免疫SPF鸡后诱导的体液免疫、CD4+/CD8+比值、外周血淋巴细胞的增殖能力和H5亚型AIV强毒攻击后的免疫保护效力。【结果】rFPVLP-△73LRH5A和rFPVLP-△214LRH5A体外诱导脾细胞产生的IFN量显著高于rFPVLP-12LSH5A,而免疫10d后的CD4+/CD8+比值显著低于rFPVLP-12LSH5A;3种重组鸡痘病毒诱导外周血淋巴细胞增殖的能力没有明显差异;3种重组病毒在SPF鸡均产生针对H5亚型AIV的HI抗体,免疫14d后rFPVLP-△214LRH5A组诱生的HI抗体水平显著低于rFPVLP-12LSH5A组的抗体,但3组在免疫21d后HPAIV的致死性攻击时,均100%被保护。【结论】鸡痘病毒ORF73和ORF214编码蛋白具有IL-18结合蛋白抑制IFN产生的功能,虽然缺失株和亲本株重组鸡痘病毒在细胞和体液免疫应答存在一定差异,但在SPF鸡均能诱导产生良好的免疫保护。