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作 者:胡月[1,2] 戚亭[2] 赵世华[2] 关平原[1] 王晓钧[2]
机构地区:[1]内蒙古农业大学兽医学院/农业部动物疾病临床诊疗技术重点实验室,内蒙古呼和浩特010018 [2]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/马传染病与慢病毒创新团队,黑龙江哈尔滨150001
出 处:《中国预防兽医学报》2014年第8期651-654,共4页Chinese Journal of Preventive Veterinary Medicine
基 金:国家科技支撑计划(2012BAD46B01-02;2012BAD46B03);公益性行业(农业)科研专项经费项目(201003075)
摘 要:为建立马动脉炎病毒(EAV)的快速检测方法,本实验以EAV N蛋白单克隆抗体(MAb)2B9为捕获抗体,辣根过氧化物酶(HRP)标记的EAV N蛋白MAb 2B3(HRP-2B3)为检测抗体,建立EAV双抗体夹心ELISA检测方法。结果显示,该方法的最佳工作条件为:MAb 2B9的包被浓度为2μg/mL,HRP-2B3的工作浓度为2μg/mL,以OD450nm≥0.124为阳性判定标准。该方法对马传染性贫血病毒、马疱疹病毒I型和IV型、马流感病毒等均无交叉反应,特异性好;最低检出限为病毒标准品200倍稀释(103.2TCID50),敏感性高。3次重复试验建立的标准曲线的相关系数(R2)均大于0.997。本实验建立的EAV双抗体夹心ELISA方法具有特异性好、敏感性高等优点,适于EAV的快速检测。To develop a method for EAV detection, a double-antibody sandwich ELISA (DAS-ELISA) was developed using MAb 2B9 against EAV nucleoprotein as capture antibody and MAb 2B3 conjugated to HRP (HRP-2B3) as detecting antibody under the optimized reaction conditions of coating with MAb 2B9 at 2 μg/well, detecting with HRP-2B3 at 2 μg/well with a cutoff value of 0.124 (OD450nm). The specificity test shown the DAS-ELISA was specifically detected EAV with a detection limit of 103.2 TCIDt0, but no crossing-reaction to equine herpes virus I, equine herpes virus IV, equine influenza virus and equine infectious anemia virus. In addition, the standard curve of EAV quantification by the DAS-ELISA had linear correlation with three times repeated tests and the R2 were above 0.997. These results demonstrated that the DAS-ELISA method was specific and sensitive, which had a potential to be applicable for the EAV detection in horse.
关 键 词:马动脉炎病毒 双抗体夹心ELISA 单克隆抗体 检测
分 类 号:S852.65[农业科学—基础兽医学]
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