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Evaluation of Enzyme-Linked Immunosorbent Assays for Detection of Mycoplasma bovis-Specific Antibody in Bison Sera

机译:酶联免疫吸附法在牛血清中检测牛支原体特异性抗体的评价

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摘要

Mycoplasma bovis has recently emerged as a significant and costly infectious disease problem in bison. A method for the detection of M. bovis-specific serum antibodies is needed in order to establish prevalence and transmission patterns. Enzyme-linked immunosorbent assays (ELISAs) validated for the detection of M. bovis-specific serum IgG in cattle are commercially available, but their suitability for bison sera has not been determined. A collection of bison sera, most from animals with a known history of infection or vaccination with M. bovis, was tested for M. bovis-specific IgG using commercially available kits as well as an in-house ELISA in which either cattle or bison M. bovis isolates were used as a source of antigen. Comparison of the results demonstrates that ELISAs optimized for cattle sera may not be optimal for the identification of bison seropositive for M. bovis, particularly those with low to moderate antibody levels. The reagent used for the detection of bison IgG and the source of the antigen affect the sensitivity of the assay. Optimal performance was obtained when the capture antigen was derived from bison isolates rather than cattle isolates and when a protein G conjugate rather than an anti-bovine IgG conjugate was used for the detection of bison IgG.
机译:牛支原体最近已成为野牛的重要且昂贵的传染病问题。需要一种用于检测牛分枝杆菌特异性血清抗体的方法,以确定流行和传播方式。经验证可检测牛中牛分枝杆菌特异性血清IgG的酶联免疫吸附法(ELISA)可商购,但尚未确定其对野牛血清的适用性。使用市售试剂盒以及内部ELISA(其中包括牛或野牛M),从大多数已知有牛分枝杆菌感染或接种史的动物的牛血清中检测牛分枝杆菌特异性IgG。牛分离株被用作抗原来源。结果的比较表明,针对牛血清进行优化的ELISA可能不是鉴定牛分枝杆菌的野牛血清反应阳性的最佳方法,尤其是那些抗体水平低至中等的牛。用于检测野牛IgG的试剂和抗原来源会影响测定的灵敏度。当捕获抗原来源于野牛分离株而不是牛分离株,并且蛋白G偶联物而不是抗牛IgG偶联物用于检测野牛IgG时,可获得最佳性能。

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