鸡传染性法氏囊病超强毒Gx与疫苗毒Gt在鸡体内的复制研究

Replication Property of Very Virulent Infectious Bursal Disease Virus Gx and Vaccine Strain Gt in Specific-pathogen-free Chicken

原文传递

导出

摘要本试验利用鸡传染性法氏囊病超强毒Gx及其致弱疫苗毒Gt为对象,研究超强毒与弱毒株在鸡体主要免疫器官内的复制情况,以探讨两类毒株表现不同生物特性的原因。分别利用鸡胚半数致死量和鸡胚成纤维细胞半数感染量对超强毒Gx和疫苗株Gt进行病毒滴度的测定;再利用荧光定量RT-PCR对两类毒株进行病毒量的校准。以相同量的病毒对2周龄SPF鸡进行攻毒。攻毒试验表明超强毒Gx能造成47.5%的死亡,法氏囊、脾脏、胸腺等免疫器官均严重损伤;而疫苗毒Gt无致死,且未能造成任何病理可见的损伤。病毒的体内复制情况表明超强毒相对于疫苗毒复制更为迅速,病毒载量更高。 To study biological characteristics of infectious bursal disease viruses, the very virulent infectious bursal disease virus （vvIBDV）Gx and vaccine strain Gt were used to compare the replication property in main immune or- gans of specific-pathogen-free （SPF）chicken. The titer of Gx was measured by 50% chicken embryo lethal dose （ELDs0） and the titer of Gt was measured by 50% tissue culture infectious dose （TCIDs0）. The viral loads of Gx and Gt were detected by realtime RT-PCR. Two-week-old SPF chickens were challenged by the same dose of Gx or Gt. The results of virus challenge assay showed that the mortality of Gx was 47.5%, and bursa, spleen and thymus were damaged severely in Gx challenge group. No deaths or any histopathological changes were obsmwed in Gt group. The data of viral replication of Gx and Gt indicated that Gx replicated faster than Gt in vivo, and higher load of virus was detected in bursa of Gx than that of Gt.

作者李久宽王永强康忠惠王琦高玉龙高宏雷祁小乐秦立廷林欢王笑梅许修宏

机构地区东北农业大学中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室/禽传染病研究室

出处《中国家禽》北大核心 2012年第1期15-18,共4页 China Poultry

基金现代农业肉鸡产业技术体系建设(nycytx-42-G3-01)

关键词传染性法氏囊病病毒超强毒疫苗毒体内复制 infectious bursal disease virus very virulent strain vaccine strain replication in vivo

分类号 S858.315.3 [农业科学—临床兽医学]

引文网络
相关文献

参考文献8

1Lu Kerr P D,Saif Y M. Infectious bursal disease[M]//Calnek B W,Barnes H T,Beard C W,et al. Disease of Poultry. 10th. Ames:Iowa State University Press,1997.
2Azad A A,Barrett S A,Fahey K J. The characterization and molecular cloning of the double-stranded RNA genome of an Australian strain of infectious bursal disease virus [J]. Virology, 1985,143:35-44.
3Kibenge F S, Qian B, Cleghom J IK. Infectious bursal dis- ease virus polyprotein processing does not involve cellular prote-ases[J]. Arch Virol, 1997,142:2401-2419.
4Mundt E,Beyer J,Muller H. Identification of a novel pro- tein in infectious bursal disease virus-infected cells[J].J Gen Vi- rol, 1995,76 : 437-443.
5Cosgrove A S. An apparently new disease of chicken-avian nephrosis[J]. Avian Dis, 1962,6 : 385-389.
6Ismail N M,Saif Y M,Moorhead P D. Lack of pathogenici- ty of five serotype Ⅱ infectious bursal disease viruses in chick- ens[J]. Avian Dis, 1988,32 : 757-759.
7Yu Wen Y Q,Gao Y L, Gao H L,et al, Sequence analysis of the VP2 hypervariable region of eight very virulent infectious bursal disease virus isolates from the northeast of China[J]. Avian Dis, 2008,52 : 284-290.
8宇文延青,高玉龙,高宏雷,祁小乐,杨金雨,王晓燕,秦立廷,林欢,李俊山,刘伟,李铁强,邓小芸,王笑梅.中国部分地区传染性法氏囊病病毒分子流病学调查[J].中国家禽,2009,31(12):11-14. 被引量：15

二级参考文献11

1刘福致周蛟刘庆新等.北京地区鸡传染性法氏囊病的初步调查.畜牧与兽医,1980,(4):25-26,48.
2毕英佐.广东地区鸡传染性囊病的研究.华南农业大学学报：自然科学版,1985,1:46-61.
3Bottcher B,Kiselev N A,Stel M V,et el. Three-dimensional structure of infectious bursal disease virus determined by electron cryomicroscopy [J]. J Virol, 1997,71 ( 1 ) : 325-330.
4Brown M D,Skinner M A. Coding sequences of both genome segments of a European 'very virulent' infectious bursal disease virus [J ]. Virus Res, 1996,40 ( 1 ) : 1 - 15.
5Yuwen Y,Gao Y,Gao H,et ol. Sequence analysis of the VP2 hypervariable region of eight'very virulent'infectious bursal disease virus isolates from the northeast of China[J].Avian Dis,2008,52(2):284-290.
6Van B T,Eterradossi N,Toquin D,et al. Infectious bursal disease(Gumboro disease)[J].Rev Sci Tech,2000,19(2) :509-543.
7Berg T P,Gonze M,Meulemans G. Acute infectious bursal disease in poultry:Isolation and characterisation of a highly virulent strain [J ]. Avian Pathol, 1991,20 ( 1 ) : 133-143.
8Eterradossi N,Amauld C,Toquin D,et al. Critical amino acid changes in VP2 variable domain are associated with typical and atypical antigenicity in very virulent infectious bursal disease viruses[J]. Arch Virol, 1998,143(8) : 1627-1636.
9Fahey K J,Mcwaters P,Brown M A,et al. Virus-neutralizing and passively protective monoclonal antibodies to infectious bursal disease virus of chickens[J]. Avian Dis, 1991,35(2) :365-373.
10Mundt E. Tissue culture infectivity of different strains of infectious bursal disease virus is determined by distinct amino acids in VP2[J].J Gen Virol,1999,80(8) :2067-2076.

共引文献14

1宋军,黄成斌,潘玲.间接ELISA检测抗传染性法氏囊病病毒抗体方法的建立[J].中国家禽,2011,34(1):15-17. 被引量：2
2吴忆春.鸡传染性法氏囊病病毒SD株毒力测定[J].动物医学进展,2011,32(2):123-125. 被引量：1
3常维山,孙静,王秀玲,张万福.近年来我国鸡肾脏疾病的流行现状与防治对策[J].中国家禽,2011,33(6):6-10. 被引量：1
4苏战强,王莉莎,郭庆勇,买买提.黑牙斯丁,左里菲亚.鸡肾型传染性法氏囊病的诊断与治疗[J].中国家禽,2011,33(18):58-59.
5高玉龙,秦立廷,王笑梅.家禽病毒性免疫抑制病流行特点与防控对策[J].中国家禽,2012,34(15):5-11. 被引量：22
6张华智,杨霖,熊忠贤,何秀苗,韦平.传染性法氏囊病病毒的分离及其VP2高变区序列的比较[J].安徽农业科学,2013,41(5):1961-1963. 被引量：2
7侯宏艳,赵瑞宏,张丹俊,朱会,胡晓苗,朱传民.4种中等毒力活疫苗对鸡传染性法氏囊病病毒超强毒株感染的免疫保护作用观察[J].动物医学进展,2013,34(12):218-221. 被引量：2
8何秀苗,陈佳,康斯那,陈盛峰,韦美萍,韦平.鸡传染性法氏囊病病毒地方流行株VP1基因片段的扩增及序列分析[J].动物医学进展,2015,36(4):19-23. 被引量：1
9孟冬霞,宇文延青,武果桃,任杰,曹水清,赵娟,孟帆,刘一飞,马政禹.山西省鸡传染性法氏囊病病毒的分离鉴定[J].动物医学进展,2016,37(10):70-74. 被引量：2
10沈巍巍,陈果,何秀苗,韦平.广西梧州地区近十年传染性法氏囊病病毒vVP2变化特征分析[J].动物医学进展,2017,38(3):32-37. 被引量：7

1王文科,陈冠春,王笑梅.鸡传染性法氏囊病超强毒901株的分离和鉴定[J].华北农学报,1994,9(3):117-121. 被引量：1
2杨发青,孙恩贵,王祥生,刘俊华.伊氏锥虫多因素致弱疫苗对家兔的免疫反应[J].中国兽医科技,1998,28(4):24-26. 被引量：2
3于海,张丽,常维山,吴洪涛.鸡传染性法氏囊病超强毒的流行特点、病因及防治对策[J].山东家禽,2003,16(12):29-30. 被引量：1
4孙淑红,张志,崔治中.鸽新城疫病毒测定方法的比较研究[J].山东畜牧兽医,2000,21(5):12-13. 被引量：1
5专家锁定禽流感病毒复制时所需基因[J].江西饲料,2008(5):43-44.
6专家锁定禽流感病毒复制时所需基因[J].河南畜牧兽医（市场版）,2008,29(7):43-43.
7专家锁定禽流感病毒复制时所需基因[J].江西饲料,2008(4):44-44.
8康忠惠,王永强,王琦,李久宽,秦立廷,高玉龙,高宏雷,祁小乐,林欢,王笑梅,许修宏.鸡传染性法氏囊病超强毒VP1基因的原核表达及兔抗血清的制备[J].中国家禽,2011,34(2):11-14. 被引量：1
9陈明生.规模牛场口蹄疫的免疫程序[J].中国畜牧兽医文摘,2016,32(5):116-116.
10万遂如.猪流感的临床症状与防控措施[J].今日畜牧兽医,2015,31(4):15-17.

中国家禽

2012年第1期

浏览历史

内容加载中请稍等...

鸡传染性法氏囊病超强毒Gx与疫苗毒Gt在鸡体内的复制研究

参考文献8

二级参考文献11

共引文献14

相关作者

相关机构

相关主题

浏览历史