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检测马传贫病毒跨膜蛋白主要免疫决定区抗体间接ELISA诊断方法的建立 被引量:1

Development of an indirect ELISA for detecting the antibody of immunodominant region of transmembrane envelope protein of EIAV
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摘要 本试验以纯化的重组马传贫病毒跨膜蛋白主要免疫决定区蛋白作为诊断抗原建立了间接ELISA诊断方法,确定其最佳工作条件为每孔包被重组抗原2μg,兔抗马IgG酶标抗体以1∶4000,血清以1∶40倍稀释,底物作用时间为10min;判定标准为P/N值大于2,且OD值大于0.2的血清为阳性,否则判为阴性。本试验所建立的诊断方法与琼扩试验以及以琼扩抗原作为包被抗原的ELISA试验进行了比较,表明该诊断方法敏感性更高。特异性和重复性试验表明该诊断方法具有良好的特异性和重复性。通过对4匹马传贫驴白细胞弱毒疫苗免疫马血清抗体的检测,发现均在接种2周后可产生抗马传贫病毒跨膜蛋白主要免疫决定区相应抗体。此抗体一直持续存在到本试验检测的免疫后17个月,且效价较高。用此方法检测203份马血清样品,其中161份呈抗体阳性,还检测了马传贫自然感染马血清93份,结果全部为阳性。 An indirect enzyme-linked immuosorbent assay (iELISA) for detecting anti-TMlR antibody has been developed by coating plate with the recombinant TMIR protein. The optimum conditions of iELISA were that the foht of the TMIR protein coated is 2μg, the rabbit anti-horse IgG conjugated with perosidase is 1:4 000, the sera are 1:40 and the reaction time of o-phenylenediamine(OPD) is 10 minutes. A positive/negative(P/N) value higher than 2.0 and OD value over 0.2 was determined as comprehensive positive standard for the ELISA. The iELISA is more sensitive compared with Agar gel immunodiffusion (AGID) and ELISA with AGID antigen. The result showed that the assay was specific and repeatable. Serum antibody of 4 horses inoculated with DLAV were detected with the iELISA. The result indicated that the 4 horses induced the antibody against TMIR 2 weeks after inoculation. The TMIR-specific antibody titer eventually reached a plateau and remained 17 months. 203 serum samples were detected by the diagnostic assay, in which 161 serum samples were positive. In addition,93 serum samples collected from EIAV-infected horses were detected with the iELISA, and the results showed that all samples were positive.
作者 朱远茂 王海燕 郭巍 李兆利 赵立平 薛飞 相文华 沈荣显
机构地区 中国农业科学院哈尔滨兽医研究所 哈尔滨医科大学实验动物中心
出处 《中国预防兽医学报》 CAS CSCD 北大核心 2006年第2期191-196,共6页 Chinese Journal of Preventive Veterinary Medicine
关键词 EIAV跨膜蛋白主要免疫决定区 ELISA 建立 TMIR of EIAV ELISA development
分类号 S852.621 [农业科学—基础兽医学]
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参考文献11

  • 1Sarah B T,Dazi R I,Vandana K,et al.Development of a fluorescence polarization-based diagnostic assay for equine infectious anemia virus[J].Journal of clinical microbiology,2000,38(5):1854-1859.
  • 2Nancy R,Louise H,Raymond C S,et al.Synthesis and processing of the trasmembrane envelope protein of equine infectious anemia virus[J].J Virol,1990,64:3770-3778.
  • 3Coggins L,Norcross N,Nusbaum S R.Diagnosis of equine infectious anemia by immunodiffusion test[J],Am J Vet Res 1972.33:11-18.
  • 4Adriana S,Veronica V,Mario R,et al.Design and validation of an ELISA for equine infectious anemia (EIA) diagnosis using synthetic peptides[J].Vet Microbiol,2001,79:111-121.
  • 5戴玉坤 宁希德 沈荣显 等.应用免疫吸附试验(ELISA)检测马传染性贫血病毒抗体的研究.中国农业科学,1984,1:81-85.
  • 6Thomas L M,Huntington P J,Mead L J,et al.A soluble recombinant fusion protein of the transmembrane envelope protein of equine infectious anemia virus for ELISA[J].Vet Microbiol,1992,31:127-137.
  • 7dos Reis J K,Melo L M,Rezende M R,et al.Use of an ELISA test in the eradication of an equine infectious anemia focus[J].Trop Anim Health Prod,1994,26(2):65-68.
  • 8Payne S L,Fang F D,Liu C P,et al.Genetic variation and lentivirus persistence:variation in envelope gene sequences during EIAV infection resemble changes reported for sequential isolates of HIV[J].Virology,1987,161:321-331.
  • 9Chong Y H,Ball J M,Issel C J,et al.Analysis of equine humoral immune responses to the transmembrane envelope glycoprotein (gp45)of equine infectious anemia virus[J].J Virol,1991,65:1013-1018.
  • 10Lew M A,Thomas L M,Huntington P J.A comparison of ELISA,FAST-ELISA and gel diffusion tests for detecting antibody to equine infectious anemia virus[J].Vet Microbiol,1993,34:1-5.

共引文献3

同被引文献20

  • 1Smith M H, Frey M L, Dierks R E. Isolation , characterization and pathogenicity studies of a bovine respiratory syncytial virus. Archives of Virology, 1975,47 ( 3 ) :237 - 247
  • 2Solis-Calderon J J, Segura-Correa J C, Aguilar-Romero F, et al. Detection of antibodies and risk factors for infection with bovine respiratory syncytial virus and parainfluenza virus-3 in beef cattle of Yucatan, Mexico. Preventive Veterinary Medicine, 2007,82(1-2) :102 - 110
  • 3Baker J C, Frey M L. Bovine respiratory syncytial virus. Vet Clinics of North America: Food Animal Practice, 1985, 1:259 - 275
  • 4Hagglund S, Hjort M, Graham D A,et al. A six-year study on respiratory viral infections in a bull testing facility. The Veterinary Journal,2007,173(3) : 585-593
  • 5Levine S, Klaiber Franco R, Paradiso P R. Demonstration that glycoprotein G is the attachment protein of respiratory syncytial virus. J Gen Virol, 1987,68:2521 - 2524
  • 6Teng M N, Collins P L. Altered growth characteristics of recombinant respiratory syncytial viruses which do not produce NS2 protein. J Virol, 1999,73:466 - 473
  • 7Taylor G, Rijsewijk F A M, Thomas L H, et al. Resistance to bovine respiratory syncytial virus (BRSV) induced in calves by a recombinant bovine herpesvirus-1 expressing the attachment glycoprotein of BRSV. J Gen Virol, 1998,79 : 1759 - 1767
  • 8Hendricks D A, Baradaran K, Mclntosh K, et al. Appearance of a soluble form of the G protein of respiratory syncytial virus in fluids of infected cells. J Gen Virol,1987 ,68 :1705 - 1714
  • 9Hendricks D A, McIntosh K, Patterson J L. Further characterization of the soluble form of the G glycoprotein of respiratory syneytial virus. J Virol, 1988,62:2228 - 2233
  • 10Roberts S R, Lichtenstein D, Ball L A, et al. The membraneassociated and secreted forms of the respiratory syncytial virus attachment glycoprotein G are synthesized from alteruative initiation eodons. J Virol, 1994,68:4538 - 4546

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中国预防兽医学报
2006年 第2期

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