Quantitative Detection of Antibodies to Aleutian Disease Virus in DriedBlood Spots as an Estimation of Hypergammaglobulinemia in Mink

Virology & mycology : infectious diseases Pub Date : 2015-11-12 DOI:10.4172/2161-0517.1000147

A. Andersson, H. B. Reineck, A. Nyman, P. Wallgren

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引用次数: 7

Abstract

Infections with Aleutian disease virus (ADV) cause a progressive hypergammaglobulinemia, immune complex formation and plasma cell infiltrations in internal organs which induce a multi-systemic disease with high mortality. Serum ADV antibodies have traditionally been diagnosed with counter immunoelectrophoresis (CIEP) as a gold standard for qualitative assessment separating infected from non-infected animals, but less laborious ELISA methods have been confirmed to be equally sensitive. A way to simplify the diagnostics further could be to demonstrate antibodies in Dried blood spot samples (DBS). However, quantitative analysis of ADV antibodies in DBS and its correlation to the degree of hypergammaglobulinemia have not been scientifically published. The aim of this paper was to describe the adaptation and validation of the VP2 ELISA to ADV antibody detection in DBS and compare the estimated antibody levels in DBS to CIEP results, the estimated antibody levels and albumin: gamma globulin ratio in serum. The VP2 ELISA worked technically well when transferred from serum to DBS with mean intra-assay and mean inter-assay coefficients of variation within ± 20%. The DBS VP2 ELISA had a sensitivity of 97.3% and specificity of 93.2% compared to CIEP. Further, we found a correlation coefficient between the level of antibodies in DBS and the A:γG ratio of -0.81. The correlation between the A:γG ratio and the OD450 value was superior in DBS compared to serum samples from the same mink with the most pronounced difference at low A:γG ratios. Our results confirmed that the VP2 ELISA could detect ADV antibodies in DBS with a high sensitivity and specificity when employing CIEP as gold standard. The antibody titers estimated with DBS VP2 ELISA were well correlated to the antibody titters and A:γG ratios in serum, and the DBS VP2 ELISA could be an applicable and preferable tool for estimating AD progression in mink.

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水貂干血斑阿留申病病毒抗体定量检测评价高γ球蛋白血症

阿留申病病毒(ADV)感染可引起进行性高γ球蛋白血症、免疫复合物形成和内脏浆细胞浸润，从而诱发高死亡率的多系统疾病。血清ADV抗体传统上是用反免疫电泳(CIEP)诊断的，作为定性评估分离感染和非感染动物的金标准，但较少费力的ELISA方法已被证实同样敏感。进一步简化诊断的一种方法可能是在干血斑样本(DBS)中证明抗体。然而，DBS中ADV抗体的定量分析及其与高丙种球蛋白血症程度的相关性尚未有科学报道。本文的目的是描述VP2 ELISA对DBS中ADV抗体检测的适应性和验证，并比较DBS中估计的抗体水平与CIEP结果，血清中估计的抗体水平和白蛋白:γ球蛋白比。VP2 ELISA从血清转移到DBS时，技术上工作良好，平均测定内和测定间变异系数在±20%以内。与CIEP相比，DBS VP2 ELISA的敏感性为97.3%，特异性为93.2%。此外，我们发现DBS中抗体水平与a:γG比值的相关系数为-0.81。与同一水貂的血清样品相比，DBS中A:γG比值与OD450值的相关性较好，在低A:γG比值时差异最显著。结果表明，以CIEP为金标准，VP2 ELISA检测DBS中ADV抗体具有较高的灵敏度和特异性。DBS VP2酶联免疫吸附测定的抗体滴度与血清中抗体滴度和A:γ - g比值具有良好的相关性，因此DBS VP2酶联免疫吸附测定可作为水貂AD病情发展的一种较好的预测工具。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Virology & mycology : infectious diseases

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