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用于定量检测多物种血清中抗狂犬病免疫球蛋白的阻断 ELISA 的优化和验证。

Optimization and validation of a blocking ELISA for quantitation of anti-rabies immunoglobulins in multispecies sera.

机构信息

UNL, CONICET, FBCB (School of Biochemistry and Biological Sciences), CBL (Biotechnological Center of Litoral), Ciudad Universitaria, Ruta Nacional 168 - Km 472.4 - C.C. 242, S3000ZAA, Santa Fe, Argentina.

Departamento de Rabia y Enfermedades de Pequeños Animales, Coordinación de Virología, Dirección de Laboratorio Animal (DLA)-DILAB, Servicio Nacional de Sanidad y Calidad Agroalimentaria (SENASA), Talcahuano 1660 (1640) Martínez, Buenos Aires, Argentina.

出版信息

Appl Microbiol Biotechnol. 2020 May;104(9):4127-4139. doi: 10.1007/s00253-020-10490-6. Epub 2020 Mar 13.

DOI:10.1007/s00253-020-10490-6
PMID:32170383
Abstract

We developed a fast, rabies virus-free, in vitro method, based on a blocking ELISA (bELISA), to detect and accurately quantify anti-rabies glycoprotein antibodies in serum of several animal species. In this method, purified rabies virus-like particles (VLPs) are used as antigen to coat the plates, while the presence of specific rabies immunoglobulins is revealed through blocking the recognition of these VLPs by a biotinylated monoclonal antibody. A quality by design approach was carried out in order to optimize the method performance, improving the sensitivity and, thereby, reducing the limit of detection of this assay. After the method validation, we confirmed that the bELISA method is able to detect a concentration of 0.06 IU/mL rabies immunoglobulins, titer lower than the 0.5 IU/mL cutoff value established as indication for correct vaccination. Further, we assessed the correlation between bELISA, the MNT, and the Platelia methods, confirming the accuracy of this new assay. On the other hand, precision was evaluated, obtaining acceptable repeatability and intermediate precision values, showing that this bELISA could be proposed as a potential alternative method, replacing the gold standard techniques in vaccination schemes and becoming a routine control technique within regional rabies surveillance programs.

摘要

我们开发了一种快速、无狂犬病病毒的体外方法,基于阻断 ELISA(bELISA),用于检测和准确定量几种动物血清中的抗狂犬病糖蛋白抗体。在该方法中,纯化的狂犬病病毒样颗粒(VLPs)用作包被板的抗原,而特异性狂犬病免疫球蛋白的存在则通过阻断生物素化单克隆抗体对这些 VLPs 的识别来揭示。进行了质量源于设计方法,以优化方法性能,提高灵敏度,从而降低该检测方法的检测限。方法验证后,我们证实 bELISA 方法能够检测到 0.06 IU/mL 狂犬病免疫球蛋白的浓度,效价低于作为正确接种指示的 0.5 IU/mL 截止值。此外,我们评估了 bELISA、MNT 和 Platelia 方法之间的相关性,证实了这种新检测方法的准确性。另一方面,评估了精密度,获得了可接受的重复性和中间精密度值,表明这种 bELISA 可以作为一种潜在的替代方法,替代疫苗接种方案中的金标准技术,并成为区域狂犬病监测计划中的常规控制技术。

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