猪细小病毒病血清抗体VP2-ELISA检测方法的建立  

Establishment of the Indirect ELISA for the Detection of Viral structural protein Antibodies against Porcine Parvovirus

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作  者:周洁[1,2] 南文龙[2] 何远清[1] 殷黎静[1] 任倩[1] 秦立得[2] 陈义平 

机构地区:[1]江苏大学实验动物中心,江苏镇江212013 [2]中国动物卫生与流行病学中心诊断试剂室,山东青岛266032

出  处:《现代畜牧兽医》2016年第4期1-7,共7页Modern Journal of Animal Husbandry and Veterinary Medicine

摘  要:利用纯化的猪细小病毒VP2蛋白为抗原,建立检测猪细小病毒血清抗体的间接VP2-ELISA。最佳反应条件为:抗原包被浓度300 ng/孔,4℃过夜,待检测血清1:50稀释。与猪细小病毒病阳性血清呈阳性反应,与猪瘟、猪伪狂犬病、猪繁殖与呼吸综合征、猪日本脑炎和猪圆环病毒病等5种疾病的阳性血清均无交叉反应。批间、批内试验变异系数均小于10%。用该方法与Ceditest PPV猪细小病毒抗体检测试剂盒对102份血清进行平行检测和比较,间接VP2-ELISA的敏感性为93.8%,特异性为81.1%,符合率为89.2%。结果表明,猪细小病毒血清抗体间接VP2-ELISA检测方法具有较高的敏感性和特异性,且重复性好,可用于猪细小病毒感染的血清抗体检测。In order to detect porcine parvovirus antibodies, an indirect ELISA was established, by using the recombinant VP2 protein as antigen. The reaction conditions of the VP2-ELISA were explored and optimized. The optimal coating concentration was 300 ng per well, the coating condition was at 4℃ overnight, and serum samples were diluted to 1:50. The results showed the VP2-ELISA assay was able to detect PPV positive serum, and had no cross-reactivity with serum against HCV, PRV, PRRSV, JEV and PCV, respectively. The intra and inter-assay coefficients of variation (CV) of the VP2-ELISA were all less than 10%. 102 swine serum samples were detected by the VP2-ELISA and Ceditest PPV ELISA Kit in parallel. The sensitivity and specificity of the VP2-ELISA were 93.8% and 81.1% respectively. The coincidence rate between these two assays was 89.2%. The results indicated that the indirect VP2-ELISA was highly sensitive and specific, and could be used for clinical detection of PPV antibodies.

关 键 词:猪细小病毒 抗体 VP2-ELISA 

分 类 号:S852.65[农业科学—基础兽医学]

 

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