鸡传染性法氏囊病病毒SD株毒力测定

从一个免疫失败鸡场中分离到一株鸡传染性法氏囊病病毒野毒株,命名为SD株.经血清学试验、鸡胚接种、病毒形态观察等证实了分离物为鸡传染性法氏囊病病毒(IBDV).测定病毒效价ELD50达到10-6.5/0.2 mL;动物回归试验表明,该SD株接种4周龄鸡后引起鸡群发病率为100%,病死率达85%,剖检可见法氏囊呈"紫葡萄样...     

鸡传染性法氏囊病病毒秦皇岛株的分离鉴定

将秦皇岛某养鸡场疑似为传染性法氏囊病的病死鸡进行剖检,为了对该疑似病例进行确诊,并进行流行病学研究,经对流免疫电泳,对采集的病料进行病毒的分离,阳性法氏囊病料进行病毒RNA的提取,采用套式RT-PCR对病毒的VP2高变区进行扩增,分析氨基酸序列。结果表明,该分离株为传染性法氏囊病病毒(IBDV),被检毒株与GenBank报道的标准超强毒株OKYM、UK661、DV86同源性高达100%,与V3、V2亲缘关系较近。动物回归试验可使健康鸡100%发病,病死率80%。表该分离株为鸡传染性法氏囊病病毒超强毒株。     

鸡传染性法氏囊病病毒弱毒株在鸡体连续传代后毒力增强的分子机理研究

将两株鸡传染性法氏囊病病毒（IBDV）弱毒株在SPF鸡体内连续传代至第5、第6代时,出现明显的法氏囊萎缩和B：B指数下降,表明IBDV弱毒株在鸡体内连续传代后毒力增强。为进一步阐释哪些基因位点导致了上述毒力的变化,本试验测定了基础弱毒株及其在鸡体内传代后各个代次毒的基因组序列,比对分析后发现VP2蛋白253位氨基酸发生了由H到Q或N的变异,表明VP2蛋白253位氨基酸的替换可能会增强传染性法氏囊病病毒在鸡体内的致病性。     

传染性法氏囊病毒分子鉴定及序列分析

传染性法氏囊病(Infectious bursal disease,IBD)是由传染性法氏囊病病毒(Infectious bursal disease virus,IBDV)引起的鸡和火鸡的一种急性、高度接触性传染病。本实验从山西省不同地区疑似法氏囊病鸡中分离到法氏囊病毒,经鸡胚培养繁殖、电镜观察、提取RNA、设计引物、c DNA的PCR扩增、电泳、测序。通过序列分析比对,最后鉴定其为传染性法氏囊病毒株。     

鸡传染性法氏囊病毒新型变异株的分离鉴定

本研究通过病毒分离、RT-PCR和测序分析等方法,从广东某肉鸡场发生法氏囊和胸腺严重萎缩的鸡群中分离了1株传染性法氏囊病毒,命名为GD2020株。氨基酸序列分析结果显示,分离株VP2基因高变区与近期国内分离的法氏囊病毒新型变异株SHG115株同源性为99.1%,与早期变异株Variant E株同源性为97.5%,与经典毒株、超强毒株和弱毒株同源性在89.3%～94.1%之间。进化分析结果表明,GD2020株与SHG115株属于同一分支,与早期变异株和经典毒株亲缘关系较远。GD2020株感染不引起鸡只死亡和出现腿肌出血等典型临床症状,但能引起法氏囊严重萎缩。本研究为广东地区传染性法氏囊病的防控提供了数据支持。     

传染性法氏囊病病毒强毒株HB／11的分离与鉴定

2011年8月,从河南省疑似传染性法氏囊病鸡群采集病料,通过鸡胚接种、琼脂扩散试验和RT-PCR等方法,证实分离的病毒为传染性法氏囊病病毒（Infectiousbursaldiseasevirus,IBDV）,命名为HB／11株。序列分析表明,HB／11株VP2基因的核苷酸序列与GenBank中发表的部分国内外IBDV超强毒株VP2基因序列相似性在99％左右;HB／11株VP2高变区基因含有七肽基序为SWSASGS,在222、253、256、279、284、294和299位上的氨基酸残基分别是A、Q、I、D、A、I和S,具有IBDV强毒的分子特征。动物回归试验表明,30日龄鸡群接种该毒株后引起鸡群发病率为100％,死亡率为70％,剖检可见鸡传染性法氏囊病典型病变。因此该病毒为IBDV强毒株。     

外源病毒检验用抗鸡传染性法氏囊病病毒特异性血清的制备与检定

为制备外源病毒检验用抗鸡传染性法氏囊病病毒(Infectious Bursal Disease Virus,IBDV)的特异性血清,对300只3~4周龄的SPF鸡进行了基础免疫和加强免疫。最后一次免疫后21d采血并分离血清,血清经混合、分装、冷冻真空干燥后,对其进行了无菌检验、外源病毒检验、剩余水分测定、中和效价测定和特异性检验。结果表明,本研究制备的抗IBDV特异性血清无菌检验、外源病毒检验和剩余水分测定均符合《中华人民共和国兽药典》三部(二〇一〇年版)规定;血清中和效价为1:5747,与IBDV B87株毒种中和指数为104.3,与鸡新城疫病毒La Sota株、鸡传染性支气管炎病毒H120株、鸡传染性支气管炎病毒H52株、鸡传染性喉气管炎病毒、鸡痘病毒、禽呼肠孤病毒S1133株的中和指数均不大于10,通过AGP、ELISA、HI等试验确定血清中不含其他禽源外源病毒抗体。本研究为鸡传染性法氏囊病活疫苗或毒种的外源病毒检验提供了具有良好特异性和高效价的中和用血清。     

鸭传染性法氏囊病病原分离鉴定及防治试验

从疑似鸭传染性法氏囊病的病例中分离到 １ 株鸭传染性法氏囊病毒,该病毒可使 ７ 日龄健康鸭 １００％ 发病,发病鸭具有鸭传染性法氏囊病的典型病变,用鸡传染性法氏囊高免卵黄抗体预防和治疗鸭传染性法氏囊病取得了满意效果。     

鸡传染性法氏囊病及其综合防控措施

鸡传染性法氏囊病是由传染性法氏囊病毒引起的一种急性、接触性、免疫抑制性疾病,该种疾病能够继发感染多种细菌性和寄生虫疾病。在临床上该种疾病以严重腹泻,肌肉震颤,极度衰弱为主要特征。这几年,随着鸡养殖产业不断向着集约化和规模化方向发展,鸡传染性法氏囊病和以往相比发生了显著的变化,防治难度越来越大。出现这种情况,主要是因为法氏囊病毒变异株和超强毒株的出现和扩散,再加上免疫不当等因素,使得鸡传染性法氏囊病的流行呈现新的特点。笔者主要就一起鸡传染性法氏囊病的诊断和综合防控进行分析。     

法氏囊病病毒的免疫原性

传染性法氏囊病是青年鸡的一种以免疫抑制为特征的疾病,它能引起法氏囊的严重病变。这种病是由双股双片段RNA病毒引起的,该病毒是双股RNA病毒科的一个成员。传染性法氏囊病的控制途径主要是用减毒或灭活苗免疫鸡群。在美国和欧洲认为法氏囊病毒有两种血清型,但只有血清I型病毒用于制备商品性疫苗,血清Ⅱ型病毒无致病性。最近有报道,从患有法氏囊病且有高水平抗体的鸡中分离出一株血清I型法氏囊病病毒,这一株病毒是法氏囊病病毒的变异株。有人认为具有不同抗原性的法氏囊病病毒变异毒株的出现是疫苗免疫失败的主要原因。     

传染性法氏囊病病毒株VP2基因在重组腺病毒中的表达

用RT-PCR方法从传染性法氏囊病(IBD)免疫预防失败的病鸡法氏囊组织AH1与AH2中扩增传染性法氏囊病病毒(IBDV)VP2基因。序列分析结果显示,AH1与AH2病毒VP2基因长度均为1350nt,编码450aa,核苷酸和氨基酸序列的同源性分别为98.2%、99.3%,七肽基序均为SWSASGS,在222、253、256、279、284、294和299位上的氨基酸残基分别是A、Q、I、D、A、I和S,具有IBDV强毒的分子特征。进一步将VP2基因克隆入人5型腺病毒穿梭载体(pShuttle-CMV),与腺病毒骨架载体(pAdEasyTM)共转化大肠杆菌BJ5183进行同源重组并转染HEK-293A细胞,经多次亚克隆获得了重组腺病毒rAd-(IBDV)VP2。利用Western-blot、IFA等方法检测IBDVVP2蛋白的体外表达情况,结果证明VP2基因在腺病毒中获得了表达。     

Pathogenicity and molecular analysis of an infectious bursal disease virus isolated from Malaysian village chickens

The characteristics of the pathogenic infectious bursal disease virus (IBDV) that infected avian species other than commercial chickens were largely unknown. In this study, by using in vivo and molecular methods, we had characterized an IBDV isolate (named 94268) isolated from an infectious bursal disease (IBD) outbreak in Malaysian village chickens--the adulterated descendant of the Southeast Asian jungle fowl (Gallus bankiva) that were commonly reared in the backyard. The 94268 isolate was grouped as the very virulent IBDV (vvIBDV) strain because it caused severe lesions and a high mortality rate in village chickens (>88%) and experimentally infected specific-pathogen-free chickens (>66%). In addition, it possessed all of the vvIBDV molecular markers in its VP2 gene. Phylogenetic analysis using distance, maximum parsimony, and maximum likelihood methods revealed that 94268 was monophyletic with other vvIBDV isolates and closely related to the Malaysian vvIBDV isolates. Given that the VP2 gene of 94268 isolate was almost identical and evolutionarily closely related to other field IBDV isolates that affected the commercial chickens, we therefore concluded that IBD infections had spread across the farm boundary. IBD infection in the village chicken may represent an important part of the IBD epidemiology because these birds could harbor the vvIBDV strain and should not be overlooked in the control and prevention of the disease.     

鸡传染性法氏囊病病毒VP3蛋白的原核表达及其B细胞抗原表位鉴定

为鉴定鸡传染性法氏囊病病毒(IBDV)VP3蛋白中的B细胞抗原表位,本研究将IBDV的VP3基因亚克隆于pET-28a中,构建了表达重组质粒pETVP3,经IPTG诱导在E.coli BL21(DE3)中表达了重组蛋白(rVP3).Western blot鉴定表明,rVP3能被IBDV抗血清特异性识别.同时,根据IBDV VP3的氨基酸序列,合成覆盖VP3全序列的重叠多肽,并与载体蛋白BSA藕联制备多肽人工结合抗原.Peptide-ELISA和Dot-ELISA检测结果表明VP3中有2个线性表位可以被已制备的单克隆抗体(MAb)识别,即~(728)PRDWDRLPYLNL~(739)和~(982)PKPKPKPNAPTQ~(993);Dot-ELISA结果显示,在VP3中还存在另外4个线性多克隆抗体识别位点:~(818)SLANAPQAGSKSQRA~(831),~(851)QREKD TIUSKKMETMGIYFATP~(872),~(876)ALNGHRGPSPGQLKYWQNTREI~(897)和~(961)QMKDLLLTAMEMK~(973).这些抗原表位的鉴定为开发IBD表位疫苗奠定了基础.     

检测传染性法氏囊病病毒VP4蛋白抗体试纸条的研制及应用

采用RT-PCR技术从滨州分离株中扩增出传染性法氏囊病病毒(infectious bursal disease virus,IBDV)VP4基因,将VP4基因插入到pGEX-4T-1载体上构建pGEX-4T-1-VP4,诱导表达并用谷胱甘肽-S-转移酶(GST)亲和层析柱纯化得到纯化的重组VP4蛋白。以兔抗鸡IgG为胶体金标记物,以重组IBDV VP4蛋白和羊抗兔IgG为硝酸纤维素膜检测线和质控线的包被物,制备一种能检测IBDV VP4蛋白抗体的胶体金试纸条。结果表明,该试纸条检测IBDV强毒(IBDV BC6/85)免疫的血清检测线显红色,为阳性反应;检测IBDV弱毒(IBDV NB)免疫的血清、新城疫病毒(Newcastle disease virus,NDV)标准阳性血清、禽流感H5和H9标准阳性血清、传染性支气管炎标准阳性血清及0.85%生理盐水检测线不显红色,为阴性反应。该试纸条与建立的ELISA方法相比,敏感度低2个滴度;检测320份临床血清,试纸条与ELISA的符合率达99.38%。提示,该试纸条使用方便、操作简单,10 min内可以用肉眼判断结果,可为区分IBDV的强弱毒提供参考数据,具有较大的应用价值。     

三株鸡传染性法氏囊病毒弱毒株的分离与分子鉴定

本试验在江苏省鸡场分离获得3株鸡传染性法氏囊病病毒（IBDV）,采用RT—PCR法扩增VP2基因,将产物克隆入pMD18T载体,经测序,并与IBDV代表株VP2基因的高变区序列进行分析比较。结果显示,3个分离株与超强毒株、强毒株、突变株及弱毒株的核苷酸同源性在89．5％～98．9％之间,与弱毒株Cu-1和疫苗株PBG-98同源性最高,为98．9％;推导出的氨基酸序列与代表性毒株的同源性在98．2％～99．5％之间。其中,七肽区的第三个丝氨酸残基突变为精氨酸或苏氨酸,279和284位氨基酸残基突变为天冬氨酸和苏氨酸,222、294和299位氨基酸残基分别突变为脯氨酸、亮氨酸和天冬氨酸。上述试验表明3株分离株均为临床弱毒株。     

Viral genotyping of infectious bursal disease viruses isolated from the 2002 acute outbreak in Spain and comparison with previous isolates

An infectious bursal disease (IBD) outbreak occurred in the east region of Spain in the spring of 2002 and rapidly spread thorough the whole country, although proper vaccination programs were applied. In this report, 33 infectious bursal disease viruses (IBDVs) isolated from this outbreak were characterized by nucleotide sequencing of the VP2 gene hypervariable region and were compared with reference IBD strains and the 1990s Spanish IBDVs in order to determine possible emergence of IBDV isolates with modified antigenic or virulent properties. Moreover, histopathologic and immunohistochemical studies of those cases where bursal tissues were available were carried out. Of the 33 isolates, 23 were identified as very virulent IBDVs (vvIBDVs), whereas the other 10 isolates were classified as attenuated or intermediate virulence classical strains and could possibly be IBDV live vaccine strains used in the immunization of these chickens. Results of this study indicate that wIBDV isolates from the 2002 Spanish outbreak are closely related with those from the 1990s outbreak. However, acute IBD cases have not been reported in Spain during these 10 yr. Genetic, management, and environmental factors likely related with IBD reemergence in Spain are discussed. Moreover, our results indicate that good correlation exists between the IBDV subtype present in the field and the degree of lesions in bursa tissue, as well as the immunohistochemistry staining.     

传染性法氏囊病病毒VP2基因原核表达及抗原性分析

从辽宁省某鸡场分离到一株传染性法氏囊病病毒(IBDV)。以该毒株基因组核酸为模板,应用RT-PCR扩增得到VP2基因,构建表达质粒pET28a-VP2,再将其转化至大肠埃希菌BL21(DE3)用IPTG进行诱导表达。表达产物经SDS-PAGE分析在48ku处出现特异性蛋白条带;经Western blot分析VP2蛋白可以与IBDV阳性血清发生特异性反应。用VP2蛋白制备的油乳剂疫苗免疫接种SPF鸡,2周后体内可以检测到特异性抗体。证明VP2蛋白具有重要的应用价值,为IBDV基因工程亚单位疫苗的研制奠定了基础。     

Prokaryotic Expression and Bioinformatics Analysis of VP2 Gene of Infectious Bursal Disease Virus C4 Strain

This study was aimed to investigate the relationship between the virulence characteristics of infectious bursal disease virus(IBDV) C4 strain and its VP2 amino acid sequence. The RNA of IBDV C4 strain was extracted,and its VP2 gene was amplified by RT-PCR.VP2 nucleotide sequences and deduced amino acids of different virulent IBDV strains were compared. At the same time, prokaryotic expression vector pET-32a(+) was used to express the VP2 gene. The expression of recombinant VP2 protein was detected by SDS-PAGE and Western blotting. The results showed that the VP2 gene of IBDV C4 strain belonged to the very virulent infectious bursal disease virus (vvIBDV) in evolutionary relationship, the VP2 nucleotides homology between IBDV C4 strain and other vvIBDV strains were 98.1% to 98.7%, and there were no mutations in S-W-S-A-S-G-S (326-332 amino acids) and 222(A), 256(I), 294(I) and 299(S). The VP2 amino acid sequence of IBDV C4 strain was consistent with the characteristics of other vvIBDV strains. However, there were three differences amino acids sites at 201(D/G), 281(G/R) and 313(V/A) between the amino acids of the C4 strain and the very virulent strain UK661. And the change of 281(R) was in the small hydrophilic region of 279 to 290, which was related to the antigenicity of the virus; The recombinant VP2 protein molecular weight expressed in Escherichia coli BL21 was about 67 ku. This study provided a basis for further research on antigenic changes resulting from amino acid variation of 201(G), 281 (R) and 313(A). These results indicated that the VP2 gene of the IBDV C4 strain was consistent with the major characteristics of the vvIBDV strain VP2 gene. The difference of three amino acid sites in the vvIBDV strain C4 might be related to the evolution of virulence of IBDV strain in China.