Detection of Bluetongue Virus Group-specific Antigen Using Monoclonal Antibody Based Sandwich ELISA 被引量：4

Detection of Bluetongue Virus Group-specific Antigen Using Monoclonal Antibody Based Sandwich ELISA

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摘要 A monoclonal antibody (MAb) specific for the bluetongue virus (BTV) group specific antigen (VP7) was characterized for its reactivity with purified virus and recombinant BTV VP7 (rVP7) protein and its suitability for use in the sandwich ELISA.The MAb,designated as 5B5 was specific to VP7 and belongs to IgG2a subclass and was selected for the development of the sELISA in this study.The MAb had a titer of 1:25 with BTV and 1:2 with the rVP7 protein.The sELISA is based on capturing of BTV antigen with VP7 specific MAb followed by detection using BTV polyclonal antiserum raised in rabbits.The assay was evaluated with six cell culture adapted serotypes of BTV that have been isolated from India,1,2,15,17,18 and 23.The assay could detect BTV antigen as early as day 8 in blood.It was also successfully applied for the detection of BTV group specific antigen in clinical samples of blood,washed RBCs,buffy coat and plasma.A total of 102 field samples from animals,suspected of being infected with BTV,were tested and 29.42% were positive.The blood samples were also amplified in cell culture which improved the sensitivity of the assay.Results confirmed that the sELISA is rapid and specific. A monoclonal antibody （MAb） specific for the bluetongue virus （BTV） group specific antigen （VP7） was characterized for its reactivity with purified virus and recombinant BTV VP7 （rVP7） protein and its suitability for use in the sandwich ELISA.The MAb,designated as 5B5 was specific to VP7 and belongs to IgG2a subclass and was selected for the development of the sELISA in this study.The MAb had a titer of 1：25 with BTV and 1：2 with the rVP7 protein.The sELISA is based on capturing of BTV antigen with VP7 specific MAb followed by detection using BTV polyclonal antiserum raised in rabbits.The assay was evaluated with six cell culture adapted serotypes of BTV that have been isolated from India,1,2,15,17,18 and 23.The assay could detect BTV antigen as early as day 8 in blood.It was also successfully applied for the detection of BTV group specific antigen in clinical samples of blood,washed RBCs,buffy coat and plasma.A total of 102 field samples from animals,suspected of being infected with BTV,were tested and 29.42% were positive.The blood samples were also amplified in cell culture which improved the sensitivity of the assay.Results confirmed that the sELISA is rapid and specific.

作者 Pradeep Narayan Gandhale Veerakyathappa Bhanuprakash Vinayagamurthy Balamurugan Madhusudhan Hosamani Gnanavel Venkatesan Raj Kumar Singh

机构地区 Division of Virology Project Directorate on Animal Disease Monitoring And Surveillance Indian Veterinary Research Institute National Research Centre on Equines

出处《Virologica Sinica》 SCIE CAS CSCD 2010年第6期390-400,共11页 中国病毒学（英文版）

关键词 BLUETONGUE DIAGNOSIS ELISA Monoclonal antibody Sandwich ELISA 夹心ELISA 单克隆抗体蓝舌病病毒病毒检测人与生物圈计划北京电视台原基础 VP7基因

分类号 R373 [医药卫生—病原生物学]

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参考文献24

1Anderson J.Use of monoclonal antibodies in a blocking ELISA to detect group specific antibodies to bluetongue virus. Journal of Immunological Methods . 1984
2Bhanuprakash V,Hosamani M,Singh N K, et al.Comparative efficacy of indirect ELISA with competitive ELISA in the detection of bluetongue virus. Indian Journal of Animal Sciences . 2007
3Lelli R,Portanti O,Langella V, et al.Production of a competitive ELISA kit for the serological diagnosis of bluetongue disease. Vet Ital . 2003
4Orru G,Ferrando M L,Meloni M, et al.Rapid detection and quantitation of bluetongue virus (BTV) using a molecular beacon fluorescent probe assay. Journal of Virological Methods . 2006
5Portanti O,Luciani M,Ronchi G F.Rapid detection of bluetongue virus in blood and organ samples using a capture enzyme-linked Immunosorbent assay. Vet Ital . 2005
6Wuijckhuise V L,Dercksen D,Muskens J, et al.Bluetongue in The Netherlands; Description of the first clinical cases and differential diagnosis. Common symptoms just a little different and in too many herds. Tijdschrift Voor Diergeneeskunde . 2006
7Fauquet CM,Mayo MA,Maniloff J,et al.Virus Taxonomy: Eighth Report of the International Committee on Taxonomy of Viruses. . 2005
8Laemmli U K.Cleavage of structural proteins during the assembly of the head of facteriophage T4. Nature . 1970
9Reed LJ,Muench H.A simple method of estimating fifty percent endpoints. American Journal of Hygiene . 1938
10Sambrook J,Fritsch EF,Maniatis T.Molecular Cloning: A Laboratory Manual. . 1989

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7单思言.秋天的落叶[J].学生之友（小学版）,2009(23):80-80.
8王稚颖,潘红.水仙花[J].小星星（作文100分）（小学3-6年级）,2011(1):44-44.
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Detection of Bluetongue Virus Group-specific Antigen Using Monoclonal Antibody Based Sandwich ELISA 被引量：4

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