Evolutionary implications of Avian Infectious Bronchitis Virus(AIBV)analysis

为开发有效疫苗，识别变化对病毒的幸存哪个氨基酸很重要是必要的。我们在鸟的传染支气管炎病毒(AIBV ) 反调查氨基酸替换特征疫苗的 serotype (DE072 ) 和剧毒的病毒的紧张(GA98 ) 到的遗传因子的领域更好理解 AIBV 的适应进化。另外， SARS Coronavirus (SARS-CoV ) 也以一样的方法被分析。发现极端相似性在氨基酸替换模式在 AIBV 和 SARS 之间存在有趣。它建议总的来说导致的氨基酸变化残余充电变，极性应该被付特殊注意到在疫苗的发展期间。

E Protein Prokaryotic Expression of Avian Infectious Bronchitis Virus

The small envelope protein （E） gene of avian infectious bronchitis virus （IBV） M41 strain was cloned, and then it was subcloned into prokaryotic expressing vector pGEX-6P-1. The recombinant plasmid was transformed into E.coli. BL21 and induced by IPTG. SDS-PAGE result showed that when objective protein fused with GST （about 20 ku）, the relative molecular mass of fusion protein was 38 ku. It indicated that objective protein was about 12.4 ku. The result showed that E protein was expressed successfully, it was useful to the subsequent E protein research.

Isolation and Identification of Avian Infectious Bronchitis Virus

[ Objective] The aim was to isolate and identify avian infectious bronchitis virus （IBV） from diseased chickens. [ Method] IBVs were iso- lated from the diseased chickens in a chicken farm in Anhui Province with blind passage method to observe virus pathogenicity. Then animal regres- sion test was made to replicate symptoms of bronchial congestion in SPF chickens and S1 gene segments were amplified and isolated, followed by comparison with IBV vaccine strains. [ Result] Detection of Hemagglutinating activity （HA） showed that allantoic fluid had no concerning effect on erythrocyte, suggesting that NDV and AIV were not included in the isolated viruses. However, the erythrocyte could be agglutinated with allantoic fluid treated with 1% of pancreatin, which is in consistent with biological characters of IBV. After SPF chickens were inoculated with the 6^th SPF al- lantoic fluid, bronchial congestion was replicated, proving that the isolated virus was avian IBV, named IBV XZ strain. [ Conclusion] This study pro- vides a theoretical basis for prevention of avian infectious bronchitis.

The Establishment of Fluorescent PCR Detection Method for Avian Infectious Bronchitis Virus

[ Objective] The aim was to to establish a kind of peculiar, sensitive and quick fluorescent PCR detection method. [Method] A peculiar, sensitive and quick method of fluorescent PCR detection for avian infectious bronchitis virus was established, the standard curve was built, specific primers, susceptibility and repeatability was detected. [ Result] This method diagnosed avian infectious bronchitis virus peculiarly, sensitively and quickly, simple and easy to use, time short, suitable for clinical testing. [ Conclusion] This research laid the foundation to diagnose avian infectious bronchitis virus.

Cloning and Sequencing of S Gene of Novel Variant of Infectious Bronchitis Virus ZJ971 Isolates in China

A novel proventriculopathogic variant (isolate ZJ971) of infectious bronchitis virus (IBV) was identified from enlarged proeventriculus of the sick chickens in the study. The S gene cDNA segment with 3.6 kb in length was amplified by RT-PCR with special primers from the ZJ971 viral isolate of (IBV) and cloned into plasmid pBluescript SK( + ). The recombinants containing S gene of IBV-ZJ971 isolate were identified by digestion of restriction enzyme EcoRI, BamHI and PCR amplification. The cloned S gene from isolate IBV-7J971 was composed of 3492 bp in length encoding for a polypeptide of 1080 amino acids. Comparing the nucleotide of S gene of IBV isolate ZJ971 with that of reported IBV strains Beaudette, M41, Ark99 and CuT2, the homology was 97.3%, 97.5%, 88.6% and 85.6%, respectively; and the homology of the deduced amino acids of S protein of IBV isolate ZJ971 was 96%, 96.3%, 86.1% and 83.1% respectively; especially, the mutation of 3241st nucleotide of S gene of IBV isolate ZJ971 from G to T resulted in the translating termination of S protein at 3240th nucleotide site.

Prokaryotic Expression of Infectious Bronchitis Virus S1 Gene and Analysis of Biological Activity of Recombinant Protein

[Objective] To study the prokaryotic expression and antigenicity identification of S1 gene from avian infectious bronchitis virus （IBV）. [Method] The S1 gene was cloned into a pMD18-T vector to yield a recombinant plasmids pMD18-T-IBV-S1. Then S1 gene was inserted into the multiple cloning site of a prokaryotic expression vector pET-32a （ ＋ ）. The recombinant plasmid was transformed into E. coil BL21. The recombinant protein was induced by IPTG and measured by SDS-PAGE and western-blotting. [Result] The S1 gene was successfully expressed in E. coil BL21, the fusion proteins were about 66.0 kDa in a form of inclusion body. Western-blotting test showed that the recombinant proteins could be identified by IBV polyclonal antibody. [ Conclusion] The recombinant proteins of S1 gene have the antigenicity, which lays a good foundation for further research on new generation vaccine of IBV.

腺胃病变型鸡传染性支气管炎病毒分离株(IBV-D971)对SPF鸡的致病力试验

用腺胃病变型鸡传染性支气管炎病毒分离株 Ｉ Ｂ Ｖ Ｄ９７１ 毒株接种１ 日龄 Ｓ Ｐ Ｆ 鸡， 可引起６０ ％ 死亡。该毒在 Ｓ Ｐ Ｆ 鸡体传２ 代后， 接种１ 日龄 Ｓ Ｐ Ｆ 鸡， 可引起１００ ％ 死亡。对人工感染病例进行了系统的病理学观察， 主要的眼观病理变化为腺胃胃壁增厚、乳头消失或乳头扁平， 乳头顶部凹陷坏死， 肾肿大、尿酸盐沉积。主要的组织学变化为腺胃粘膜上皮坏死脱落、固有层水肿、有炎性细胞浸润、肌层有淋巴细胞浸润、肌细胞坏死、腺小叶腺细胞坏死、核浓缩。小肠粘膜绒毛上皮增生、呈复层结构、固有层水肿、有大量淋巴细胞浸润。肾间质水肿、细尿管和肾小球间质内有淋巴细胞浸润。肝、心等实质细胞变性， 以至局灶性坏死。脾、胸腺及法氏囊的淋巴组织萎缩等， 人工感染鸡病例和自然发病鸡的病理变化基本相同。

IBV广东分离株GD05 S1基因的克隆、鉴定及其表达

Acording to Avian Infectious Brochitis virus( IBV) Beaudette strain S1 gene sequence, a pair of primers were designed and synthesized. With the primers , IBV Guangdong isolation strain GD05 S1 gene was successively amplified by RT-PCR.PCR product was digested with BstY I,\%Hae\% III and \%Pst\% I respectively, the result showed RFLP pattern of was the same as that of M41 S1 gene. IBV GD05 strain was thought as Mass serotype primaryly. IBV GD05 S1 gene was cloned into pGEM-T vector and sequenced, its sequence was consisted of 1611 base pairs. By comparison , the nucleotide sequence was 97.14% identical to that of IBV M41. IBV GD05 S1 gene was subcloned into expression vector pET21d. SDS-PAGE experiment showed that it expressed in \%E.coli.\%

广西1985年～2008年IBV分离株S1基因高变区Ⅰ和N基因的序列和系统进化分析

为了解广西传染性支气管炎病毒(IBV)的纤突蛋白S1基因高变区Ⅰ(HVRⅠ)和核(N)蛋白基因变异情况及S1和N基因变异的相关性,本研究应用RT-PCR方法扩增了广西1985年～2008年的21株IBV的S1基因HVRⅠ和N基因,并进行了克隆、序列测定及分析。结果发现:广西存在着多种基因型IBV流行;广西IBV分离株S1基因存在广泛的点突变和插入现象;N基因序列存在氨基酸替代现象。21株IBV中12株在S1基因HVRⅠ和N基因遗传进化树中均归属相同群,其余毒株却归属不同的群。2005年分离的GX-NN5存在基因重组现象。以上结果表明了广西IBV毒株存在基因突变和基因重组现象,S1和N基因的变异不完全平行,有些毒株间的S1和N基因差异很大。

IBV M基因与IL-18基因共表达DNA疫苗的免疫原性

将禽传染性支气管炎病毒(IBV)的M基因和禽白介素18(IL-18)基因分别插入双顺反子质粒pIRES-EGFP/DsRed中,构建IBV M和IL-18基因的共表达质粒pIRES-M/IL18及表达M基因的pIRES-M质粒。通过脂质体转染Vero细胞,利用RT-PCR及间接免疫荧光检测质粒在体外的表达。将构建的质粒用脂质体包裹后,通过腿部肌肉多点注射免疫7日龄雏鸡,28日龄加强免疫1次;免疫前后均采血检测ELISA抗体效价和外周血CD3+、CD4+、CD8+T淋巴细胞的数量;二免后2周用IBV肾型强毒进行攻毒。结果显示,pIRES-M/IL18、pIRES-M质粒均在Vero细胞中有效地转录并表达目的蛋白。从免疫后7 d起,pIRES-M/IL18免疫组产生的抗体水平及外周血T淋巴细胞亚群数量均高于pIRES-M组。pIRES-M/IL18、pIRES-M组对强毒的攻击保护率分别为65%和40%。以上结果表明,禽源IL-18基因与IBV M基因共表达可增强鸡体对DNA疫苗的免疫应答,提高对IBV强毒的抵抗力。

引起免疫失败的IBV分离株的生物学特性及结构基因分析

本研究应用鸡胚尿囊腔接种的方法,从广西患传染性支气管炎的免疫失败的病鸡中分离到一株传染性支气管炎病毒(IBV)(命名GX-YL5),通过间接血凝试验、动物回归试验和气管环交叉中和试验对该毒株进行鉴定和主要生物学特性的研究,同时利用RT-PCR技术扩增克隆该病毒的S1基因和N基因并测定其核苷酸序列。结果表明:该病毒株有间接血凝性;致病性较强;血清型不同于常用疫苗株H120、Ma5、4/91。同源性分析表明,S1基因核苷酸和氨基酸序列与参考株的同源性分别为63.5%～81.2%和50.7%～78.8%;N基因核苷酸和氨基酸序列与参考株的同源性分别为85.7%～87.2%和89.5%～91.7%;S1基因和N基因系统进化分析表明分离株与其它参考毒株的亲缘关系较远。S1基因和N基因分型与血清学试验结果相吻合。本研究结果提示了广西分离株GX-YL5可能是一个新的变异株,这可能是目前免疫失败的重要因素,同时也为研制适合本地使用的IBV疫苗提供了科学依据和物质基础。

IBV3株分离株的血清中和试验及S1基因同源性分析

通过血清中和试验、RT-PCR、核酸序列分析和S1基因的同源性分析,表明鸡传染性支气管炎病毒(IBV)BJ9601、HN9604与M41株的血清中和效价最高,其次为H120,TJ9602与试验毒株的血清中和效价较低。BJ9601、HN9604的S1基因与H120和H52的同源性很高,与H120和H52同在一个分支,其来源与H120或H52有密切关系。TJ9602的S1基因只与LDT3的同源性达到93%,共同形成一个分支,与其他毒株的同源性均在88%以下。血清中和试验和S1基因同源性之间存在较高的相关性,但并不能达到完全的吻合,即血清中和效价最高的毒株之间S1基因的同源性并不是最高的。在GenBank中登记的IBV中国大陆分离株的S1基因可分为3个基因群,其中Ⅰ群和Ⅱ群是主要的流行毒株,共有38个分离毒株,占90.48%。

IBV地方分离株致病原性和血清学分型的比较

将 6株分离自国内不同地方的 IBV流行株分别感染 SPF鸡 ,对气管和肾脏进行系统病理观察 ,发现 6株 IBV在致病原性和组织嗜性上存在显著差异 ,其中 QD可引起严重的呼吸道损伤 ,并伴有相对较轻的肾脏损伤 ,其余 5株对肾脏损伤较为严重而对呼吸道损伤相对温和。用气管环组织培养交叉中和实验 (SN)和 SAS软件对 6株分离毒进行血清学分型研究 ,结果显示 QD株属于 M型 ,ZZ、GZ属于 T型 ,而 TJ、DL和 YC株是不同于 M和 T血清型的变异株。研究结果表明 ,不同 IBV毒株的致病原性和血清型有一定的相关性 ,同时也说明我国 IBV流行株已发生变异 ,并存在所谓肾型

Mab-ELISA对IBV毒株定性检测方法的建立与应用

针对禽传染性支气管炎病毒 (IBV)血清型众多、临床检测不易的难题 ,用我国自己研制的 2株IBV单克隆抗体 ,通过多种方法的比较与鉴定 ,建立起适用于定性检测IBV的包被鼠源IBV单抗的Mab ELISA方法 ,其操作程序是 :包被鼠源IBV单抗 -被检病毒 -鸡抗IBV高免血清 -兔抗鸡IgG (AGP效价 1∶32 ) -羊抗兔IgG -HPR ;用本方法对国内 46个IBV分离株及NDV、AIV H9N2、PPMV I等的检测 。

腺胃病变型鸡传染性支气管炎病毒(IBV-D971株)致弱的研究

将IBV_D971株病毒在SPF鸡胚上连续传至 12 0代 ,培育出了一株毒力明显减弱 ,并且具有良好免疫原性的腺胃病变型鸡传染性支气管炎病毒弱毒株 (IBV_D971株 )。IBV_D971F10 5代毒力明显下降 ,以 10 9.2 5EID50 接种 1日龄SPF鸡 5 / 5无不良反应。IBV_D971F10 5代毒连续通过 1日龄SPF鸡体 5代 ,未见毒力返强。以 10 3EID50 免疫 1日龄SPF鸡 ,攻毒后 5 / 5保护 ,对照 5 /

鸡胚气管环纤毛对不同类型AIBV毒株的敏感性

以鸡胚气管环纤毛运动作指示系统，应用鸡胚气管环组织培养不同血清型的７个标准ＡＩＢＶ毒株及５个不同致病型的分离毒株。采用５０ＣＤ５０病毒量ＩＢＶ毒株感染鸡胚气管环培养物，观察感染后不同时间气管环纤毛的存活率。结果表明，鸡胚气管环纤毛对不同血清类型的ＡＩＢＶ毒株敏感性各具特征。

鸡肾型IBV地方分离株N基因的克隆及分子遗传变异分析

用RT-PCR方法对分离于陕西省不同地区的8个鸡肾型IBV毒株的Ⅳ基因分别进行了扩增,将各扩增产物与T载体连接后,转化感受态细胞筛选阳性克隆质粒并进行基因测序,用DNAstar软件将这8个毒株与GenBank收录的7个IBV代表毒株的Ⅳ基因进行了比较分析,研究了其变异情况。结果表明,B01,YL,WH和 YX株与7株代表毒株的同源性较高,而G,BJ,WG,FF株与7个代表毒株的同源性相对较低。氨基酸推导序列比对结果表明,N蛋白突变以散在的点突变形式为主,其中46,48,50,75,78,189,232,236,237,299,301,350,366等位点容易发生突变,突变位点无明显规律性。

鸡传染性支气管炎病毒(IBV)的血清学分型研究

本文运用气管环血清中和试验对１２个ＩＢＶ毒株进行了血清型研究。以气管环纤毛运动为指示系统，以能中和２．０ｌｏｇ１０ＣＤ５０同源病毒血清效价为１个抗体单位，含２０个抗体单位的血清与等量病毒作用测定血清对纤毛运动保护百分率，以欧氏距离数字分类分型，并用ＳＰＳＳ软件聚类分型分析。结果表明ＳＡＩＢ１属Ｍ４１型，ＳＡＩＢ３属Ｔ型；ＸＪＩＢ接近Ｍ４１型，ＳＨＩＢ、ＳＡＩＢ２接近Ｔ型。ＸＪＩＢ，ＳＨＩＢ，ＳＡＩＢ２具有过渡性（变异性）特征。

RT-PCR和核酸探针在IBV检测中的应用

用ＰＣＲ和核酸探针杂交检测了３种毒株（Ｈ１２０株，Ｍ４１株，ＨＫ株）在鸡胚中的繁殖动态及人工感染鸡和自然感鸡气管粘液及肾组织内的ＩＢＶ．结果表明：在鸡胚中繁殖３种毒株ＩＢＶ（Ｈ１２０，ＨＫ，Ｍ４１），ＰＣＲ最早检出时间为２０～２４ｈ，克隆探针最早检出时间为２４～３０ｈ；用克隆核酸探针检测人工感染鸡，１２ｈ后能从肾脏中检出病毒。对７只就诊鸡的病变肾脏进行杂交检测和ＰＣＲ扩增，有５只均呈阳性反应。ＩＢＶ分离株ＨＫ株与标准株Ｍ４１株经ＰＣＲ扩增、ＨａｅⅢ和ＨｉｎｄⅢ酶切及ＲＦＬＰ分析，表明其属同一马萨诸塞血清型。ＰＣＲ和核酸杂交技术为生产上提供了直接从尿囊液和感染鸡组织中快速检测ＩＢＶ病毒及诊断ＩＢＶ的新方法，对ＩＢＶ的血清定型也有一定的实用价值。

鸡肾型IBV分离株M基因的克隆与特性分析

依据NCBI所登录的鸡传染性支气管炎病毒的M基因序列设计了一对引物,应用TRIzol试剂盒对8个肾型鸡传染性支气管炎病毒陕西地方分离株进行总RNA的提取,以所得到的RNA为模板,用RT-PCR对M基因进行扩增;其目的条带回收提纯后,与PMD18-T克隆载体进行连接,转化到DH5α宿主菌,并经药物抗性筛选、PCR及酶切鉴定,将所筛选鉴定出的阳性质粒进行测序,最后对测序结果进行分析。结果表明:陕西地方8个毒株(BJ2、FF2、YL2、B01、G5、YX、WH、WG)M基因长约为650 bp,其中YX、WH株本身无BamH 1酶切位点。WH与其它分离株的核苷酸同源性为91.8%～92.6%,而其它的分离株间的同源性为98.8%～99.8%。8个毒株与参考株的核苷酸同源性为74.9%～99.8%。其N端90 aa肽段与对照株相比,不同之处表现为高亲水性氨基酸取代低亲水性氨基酸,这会使其具有更好的抗原性。