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Antigen Recognition by Serum Antibodies in White-Tailed Deer (Odocoileus virginianus) Experimentally Infected with Mycobacterium bovis

机译:通过牛分枝杆菌感染的白尾鹿(Odocoileus virginianus)中血清抗体的抗原识别

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摘要

White-tailed deer (Odocoileus virginianus) have emerged as reservoirs of bovine tuberculosis in northern America. For tuberculosis surveillance of deer, antibody-based assays are particularly attractive because deer are handled only once and immediate processing of the sample is not required. Sera collected sequentially from 25 Mycobacterium bovis-infected and 7 noninfected deer were evaluated by enzyme-linked immunosorbent assay (ELISA), immunoblotting, and multiantigen print immunoassay (MAPIA) for immunoglobulin specific to M. bovis antigens. Various routes of experimental M. bovis infection, such as intratonsillar inoculation (n = 11), aerosol (n = 6), and exposure to infected deer (in contact, n = 8), were studied. Upon infection, specific bands of reactivity at ∼24 to 26 kDa, ∼33 kDa, ∼42 kDa, and ∼75 kDa to M. bovis whole-cell sonicate were detected by immunoblot. Lipoarabinomannan-specific immunoglobulin was detected as early as 36 days postchallenge, and responses were detected for 94% of intratonsillarly and “in-contact”-infected deer. In MAPIA, sera were tested with 12 native and recombinant antigens coated on nitrocellulose. All in-contact-infected (8 of 8) and 10 of 11 intratonsillarly infected deer produced antibody reactive with one or more of the recombinant/native antigens. Responses were boosted by injection of tuberculin for intradermal tuberculin skin testing. Additionally, three of six deer receiving a very low dose of M. bovis via aerosol exposure produced antibody specific to one or more recombinant proteins. M. bovis was isolated from one of three nonresponding aerosol-challenged deer. Of the 12 antigens tested, the most immunodominant protein was MPB83; however, a highly sensitive serodiagnostic test will likely require use of multiple antigens.
机译:白尾鹿(Odocoileus virginianus)在北美北部已成为牛结核病的储存库。对于鹿的结核病监测,基于抗体的测定法特别有吸引力,因为鹿只需要处理一次,而无需立即处理样品。通过酶联免疫吸附测定(ELISA),免疫印迹和多抗原印刷免疫测定(MAPIA)对从牛分枝杆菌感染的25头牛和7头未感染的鹿中依次收集的血清进行了牛分枝杆菌抗原特异性免疫球蛋白的评估。研究了实验性牛分枝杆菌感染的各种途径,例如扁桃体内接种(n = 11),气雾剂(n = 6)以及暴露于被感染的鹿(n = 8)。感染后,通过免疫印迹检测到对牛分枝杆菌全细胞超声处理的约24至26 kDa,约33 kDa,约42 kDa和约75 kDa的特定反应带。最早在攻击后36天就检测到了Lipoarabinomannan特异性免疫球蛋白,并且在94%的扁桃体内和“接触”感染的鹿中检测到了应答。在MAPIA中,用涂在硝酸纤维素膜上的12种天然和重组抗原测试了血清。所有接触感染(8个中的8个)和11个在扁桃体内感染的鹿中的10个产生与一种或多种重组/天然抗原具有反应性的抗体。通过注射结核菌素进行皮内结核菌素皮肤测试可增强反应。另外,六头鹿中有三头通过气溶胶暴露获得非常低剂量的牛分枝杆菌,产生了对一种或多种重组蛋白具有特异性的抗体。牛分枝杆菌是从三只无响应气雾剂攻击的鹿中分离出的。在所测试的12种抗原中,免疫力最强的蛋白是MPB83;其免疫原性最高。但是,高度敏感的血清诊断测试可能需要使用多种抗原。

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