重组辛德毕斯病毒E基因痘苗病毒的构建

为了构建表达辛德毕斯病毒E基因的重组痘苗病毒,本研究通过基因重组的方法将辛德毕斯病毒E基因及绿色荧光蛋白（enhanced green fluorescent protein,EGFP）基因分别连接至痘苗病毒转移载体pSTK,酶切鉴定得到阳性重组质粒pSTK-SINE-EGFP。采用脂质体转染的方法,将该重组质粒与痘苗病毒天坛株共转染BHK-21细胞,通过同源重组获得重组痘苗病毒。利用EGFP筛选阳性重组痘苗病毒vTTVV-SINE-EGFP,收集感染重组痘苗病毒的BHK-21细胞,SDS-PAGE电泳检测辛德毕斯病毒E基因在细胞中的表达情况,Western blot分析表达产物的免疫原性。结果证明辛德毕斯病毒E基因能在重组痘苗病毒vTTVV-SINE-EGFP中获得表达,且表达产物具有良好的免疫原性。表达辛德毕斯病毒E基因的重组痘苗病毒的成功构建,为研制辛德毕斯病毒活载体疫苗奠定了基础。     

H9N2亚型流感病毒光动力失活的超微结构

使用H9N2亚型流感病毒作为系统模型,用不同浓度(2,4μmol/L)的光敏剂经激光照射(12 J/cm²,20 min),使病毒颗粒失活后,使用透射电子显微镜(TEM)观察病毒粒子形态,并对病毒的感染性进行测定。结果显示,低浓度光敏剂处理组的病毒粒子膜结构虽然保持完整性,但表面糖蛋白缺失,同时丧失了对MDCK细胞的感染性;高浓度光敏剂处理组的病毒粒子膜结构不完整,出现不同程度的膜结构损伤,病毒粒子对MDCK细胞无感染性。本试验为流感病毒的光动力失活提供了可靠的试验依据。     

Lack of detection of feline leukemia and feline sarcoma viruses in diffuse iris melanomas of cats by immunohistochemistry and polymerase chain reaction.

Diffuse iris melanoma was confirmed by light-microscopic examination in 10 formalin-fixed, paraffin-embedded globes from 10 cats. To determine if feline leukemia virus or a replication defective feline leukemia virus, feline sarcoma virus, was present in these anterior uveal melanomas, immunohistochemistry and polymerase chain reaction for feline leukemia virus were utilized. Immunohistochemical staining for feline leukemia virus glycoprotein 70 was performed on all 10 tumors using an avidin-biotin complex technique. The DNA was extracted from each specimen and a 166-base pair region of the feline leukemia virus long terminal repeat was targeted by polymerase chain reaction. Immunohistochemical staining for feline leukemia virus glycoprotein 70 and polymerase chain reaction amplification of a feline leukemia virus long terminal repeat region were negative in all cases. Feline leukemia virus/feline sarcoma virus was not detected in any neoplasms and therefore was unlikely to play a role in the tumorigenesis of these feline diffuse iris melanomas.     

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。     

Isolation and preliminary characterization of an orbivirus of the Palyam serogroup from biting midge Culicoides oxystoma in Japan

An orbivirus of the Palyam serogroup was isolated from Culicoides oxystoma collected in a cowshed in Kagoshima, Southern Kyushu Island, Japan. This is the first isolation of an orbivirus of the Palyam serogroup in Japan. The virus was a spherical non-enveloped RNA virus, approximately 60 nm in diameter. The virus was resistant to ethyl ether, sodium deoxycholate and freezing-thawing, but readily inactivated by trypsin. The virus was not stabilized by 1 M MgCl2, was labile at pH 3.0 and was not precipitated by protamine sulfate. Indirect immunofluorescent staining of infected Vero cells indicated the virus to be antigenically related to D'Aguilar and Bunyip Creek viruses of the Palyam serogroup. Neutralization tests showed the virus to have no relationship with D'Aguilar virus, but to have a one-way cross-reaction with Bunyip Creek virus. The virus was tentatively designated as Kagoshima virus. A serological survey indicated dissemination of the virus in cattle populations in Kagoshima Prefecture.     

金丝雀痘诊断与痘病毒致弱试验

本试验对送检的金丝雀经实验室诊断，确认为金丝雀痘，对分离的痘病毒进行动物致病性试验、病毒分离传代和致试验、致弱毒保护力试验和返强试验。结果表明：金丝雀痘病毒经鸡胚盲传３后能适鸡胚并致死金丝雀，８代后无致病性，１３例毒性快速通过本动物３次无返强现象，金丝雀用第１３代毒刺种３０天能抵抗强毒攻击。     

Serologic detection and practical consequences of antigenic diversity among bovine viral diarrhea viruses in a vaccinated herd.

Samples of sera were obtained from 5,725 cows in a semiclosed herd. In each of the preceding 7 years, the herd was vaccinated against bovine viral diarrhea (BVD) with killed virus. Neutralizing antibody tests were done on all samples of sera, using cytopathic virus, BVD-TGAC virus, that was antigenically distinct from the vaccine virus. Most samples of sera had high titers of neutralizing antibodies against BVD-TGAC virus. In 48 samples of sera, neutralizing antibodies were not detected against BVD-TGAC virus, but were detected against the vaccine virus. Neutralizing antibodies against selected noncytopathic BVD viruses were not detected in several samples of serum that had neutralizing antibodies against the vaccine virus and BVD-TGAC virus. Noncytopathic BVD virus was isolated from sera obtained from 3 cows less than 4 years old. Two cows were available for further testing, and persistent infection with BVD virus was confirmed in both cows. The BVD viruses isolated from those cows were not neutralized by several samples of sera. Immunoprecipitation of polypeptides induced by the vaccine virus was done with selected samples of serum. Two patterns of immuno-precipitated viral-induced polypeptides were identified. One pattern was consistent with exposure of cows with live virus. The other pattern was consistent with exposure of cows with only the killed virus vaccine.     

基孔肯亚病毒和辛德毕斯病毒检测基因芯片的建立

根据GenBank中收录的基孔肯亚病毒和辛德毕斯病毒基因的保守序列,合成2种病毒E基因序列及引物,设计针对2种病毒的寡核苷酸探针,制备基孔肯亚病毒与辛德毕斯病毒特异性检测基因芯片,并对该芯片的灵敏性、特异性和重复性进行了验证。结果显示,所建立基因芯片检测方法的灵敏度是普通PCR方法的100倍。利用所制备的基因芯片,能检测到基孔肯亚病毒和辛德毕斯病毒特异性杂交信号,阴性对照病毒（基因Ⅰ型流行性乙型脑炎病毒,基因Ⅲ型流行性乙型脑炎病毒,猪繁殖与呼吸综合征病毒及流感病毒）均无杂交信号。本试验初步建立了基孔肯亚病毒与辛德毕斯病毒特异性基因芯片检测方法,该方法灵敏度高、特异性强,适用于基孔肯亚病毒与辛德毕斯病毒的流行病学调查和种特异性鉴定。     

H3亚型猪流感病毒分离与鉴定

从东莞和鹤山等地不同猪场采集的40份鼻拭子或病死猪的肺、气管病料中分离到4株有血凝活性的病毒,其中3株病毒与新城疫病毒阳性血清的HI试验为阳性,另外1株病毒与抗猪流感H3亚型猪流感病毒阳性血清的HI试验为阳性;根据猪流感病毒M基因设计引物,扩增出预期的约315 bp片段,表明该病毒为H3亚型猪流感病毒。     

Isolation of a paramyxovirus from the cerebrospinal fluid of a dog with posterior paresis

A paramyxovirus was isolated from cerebrospinal fluid of a dog with a history of incoordination and posterior paresis. The virus apparently was not related to canine distemper virus (CDV), considering the lack of virus neutralization with CDV-specific antibody, negative immunofluorescence with CDV-specific conjugate, and avirulence for ferrets. The virus was antigenically related to a prototype strain of canine parainfluenza virus, as determined by positive immunofluorescence with canine parainfluenza virus-specific conjugate and virus neutralization tests.     

猪流行性腹泻病毒变异株CH/GX/750A/2015在Vero细胞上转瓶培养条件的优化试验

本研究旨在确定猪流行性腹泻病毒（PEDV）变异株CH/GX/750A/2015株在Vero细胞上转瓶培养的最佳条件，为大规模生产高效PEDV变异株疫苗提供技术支撑。试验以10 L转瓶培养病毒，对接毒时细胞维持液中胰酶浓度（0、2、4、6、8和10 μg/mL）、细胞密度（40%、60%、80%、100%、200%）、接毒剂量（MOI分别为1、0.1、0.01和0.001）、吸附时间（0、30、60、90、120、240 min）、收毒时间（接毒后12、24、36、48、60、72 h）、维持培养温度（35、36、37和38 ℃）和转瓶转速（6、8、10、12、14、16 r/h）7个条件进行优化。结果显示，PEDV CH/GX/750A/2015株在10 L转瓶中的最佳培养条件为：细胞刚铺满单层时接毒，接毒量为MOI=0.01，维持液（无血清DMEM培养液）中胰酶质量浓度为6 μg/mL，不需吸附，维持培养温度为37 ℃，12 r/h 旋转培养48 h后收获病毒液可获得较高效价的病毒液，效价可稳定达到10^6.50 TCID₅₀/0.1 mL。本试验为 PEDV 变异株大量培养提供了参考，为变异株疫苗研发奠定了基础。     

1株牛传染性鼻气管炎病毒的分离鉴定

在对进口种用奶牛隔离检疫期间,从1头IBRV中和抗体阳性奶牛中分离出1株病毒。该分离株表现类似于IBRV特征的细胞病变,细胞圆缩,聚集成葡萄串样群落,在单层细胞上形成空洞。用特异性抗IBRV阳性血清与其进行中和试验,发现IBRV标准阳性血清对分离株的中和抗体滴度为27,与IBRV标准株的中和抗体滴度相差不到1个滴度。用OIEV推荐的IBR特异性引物对分离病毒进行PCR扩增,获得与设计基因片段大小一致的特异性条带,表明分离到的病毒为IBRV。     

RT-PCR快速诊断禽流感

根据禽流感病毒ＮＰ基因的序列分析结果,设计了一对ＮＰ基因特异的引物。采用该对引物,不经病毒分离,直接从禽流感病毒感染鸡的气管、泄殖腔棉拭子和组织样品中提取核酸, ＲＴ～ＰＣＲ可以扩增出 ３２６ｂｐ的 ＮＰ基因片段。采用该技术对１４个亚型禽流感病毒标准参考株,４个亚型１２株国内分离野毒株,ＲＴ－ＰＣＲ检测的结果都呈阳性;对新城疫病毒、传染性法氏囊病毒、传染性支气管炎病毒、传染性喉气管炎病毒以及减蛋综合症病毒,ＲＴ－ＰＣＲ扩增结果都呈阴性。禽流感病毒 Ａ／Ｇｏｏｓｅ／Ｇｕａｎｇｄｏｎｇ（Ｈ５Ｎ１）和 Ａ／Ａｆｒｉｃａｎ　Ｓｔａｒｌｉｎｇ／Ｅｎｇｌａｎｄ（Ｈ７Ｎ１）实验感染鸡样品 ＲＴ－ＰＣＲ检测与鸡胚病毒分离阳性率分别为３４／４２、３２／４２; ２４／５５、２４／５５, 二者符合率大于９５％。 ＲＴ－ＰＣＲ最少可检测到１０ｐｇ的病毒核酸。对山东某地发病鸡场样品进行ＲＴ－ＰＣＲ检测,只用６个小时就可得出准确的诊断结果,证明ＲＴ－ＰＣＲ检测方法敏感特异,可用于禽流感的快速诊断。     

Routine titration of foot-and-mouth disease virus suspensions by analytical ultracentrifugation 2nd communication: sedimentation equilibrium method.

A routine method for the determination of the virus concentration in FMD virus cultures and vaccines was developed. This method was based on sedimentation equilibrium in the analytical ultraviolet scanning ultracentrifuge. The virus suspension was first clarified. The virions were then sedimented in a preparative ultracentrifuge. The resuspended virions were diluted in a Cesium chloride solution and brought to equilibrium in the density gradient generated in the analytical ultracentrifuge. The optical density of the virus band was measured by the UV scanning system. A calculation procedure was developed to compute the density at the limits and at the maximum of the virus band. The virus concentration expressed as weight, was calculated for the original virus suspension.     

Enterovirus Neutralizing Activity in the Gastrointestinal Tract of Piglets

Neutralizing activity against porcine enterovirus strain T80 was demonstrated in the contents of the stomach, duodenum or ileum of four piglets which were suckling dams whose milk contained neutralizing substances against the same virus. No neutralizing activity was detected in the gastrointestinal contents of an unsuckled piglet or in four weaned piglets. Extracts of intestinal tissue from each of the above piglets failed to neutralize the virus. Four weaned piglets were dosed orally with live T80 virus. From nine days after infection virus neutralizing activity was found in extracts of tissue prepared from the duodenum, jejunum, ileum, caecum and colon but not in the contents of the gastrointestinal tract and a serological response to the virus was demonstrated. No virus neutralizing activity was detected in gastrointestinal tissue or contents from four weaned piglets inoculated parenterally with live T80 virus or in four piglets dosed orally with inactivated T80 virus and these piglets did not respond serologically to the virus.     

鹅细小病毒灭活疫苗种子批建立

为保证制苗所用毒种质量和稳定性,在对制苗毒种病毒含量、病毒纯净性、特异性、免疫原性及扩繁代次等研究的基础上,建立了鹅细小病毒灭活疫苗毒种种子批。试验使用鹅胚对鹅细小病毒YA98株进行了20次传代。传代毒种的鉴定结果表明:抽检的各代次的毒种均无细菌、支原体、外源病毒污染,且病毒含量检测稳定,每0.3 m L含104.78~4.85ELD50;各代次特异性检测均能被鹅细小病毒抗血清中和;将各代次病毒液制成灭活疫苗,免疫成鹅后均能产生完全保护。以此为依据,最终确定原始毒种和基础毒种的扩繁代次宜控制在5代以内,生产毒种的最高扩繁代次宜控制在15代以内。种子批的建立,为鹅细小病毒灭活疫苗的生产奠定了基础。     

Interaction of an intranasal combined feline viral rhinotracheitis, feline calicivirus vaccine and the FVR carrier state

Eight cats were vaccinated intranasally with a combined feline calicivirus/feline viral rhinotracheitis (FVR) virus commercial vaccine. Following intranasal challenge with a field strain of FVR virus and subsequent treatment with corticosteroid, no virus was recovered from any of the eight cats, while FVR virus was recovered following corticosteroid treatment from two of four unvaccinated and challenged controls. No evidence was found for the development of an FVR virus carrier state with the intranasal vaccine virus.     

The protective effect of two porcine enterovirus vaccines in swine.

The virus neutralizing substance in the gastrointestinal tract of swine vaccinated in different ways with porcine enterovirus strain T80 was characterized by tests for enhancement and absorption of virus neutralizing activity by class specific antiporcine Ig antisera. The gastrointestinal virus neutralizing activity of piglets which were vaccinated with live virus orally resided predominantly in the IgA class, although some activity was present also in the IgM and IgG classes. The serum virus neutralizing activity of this group was present in all three classes but primarily in the IgG class. The IgA in the serum of this group was presumably of gut origin. However, in piglets vaccinated with live virus intramuscularly, with formaldehyde-inactivated virus orally or intramuscularly or with ethylenimine-inactivated virus by both oral and subcutaneous routes, both serum and gastrointestinal virus neutralizing activity were attributable predominantly to antibodies of the IgG and IgM classes. None possessed serum IgA. There was evidence also for the presence of Ig fragments in some gastrointestinal extracts.     

狂犬病毒中和抗体检测试验中病毒回归试验的重要性

狂犬病毒中和试验的病毒回归试验表明,病毒攻毒液的实际剂量与理论剂量不完全一致.建议在新版<中华人民共和国兽用生物制品质量标准>中增加对病毒攻毒实际剂量范围的规定,以使结果的判定更为合理.