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使用双位点酶免疫测定法检测培养衍生的牛巴贝斯虫外抗原。

Detection of culture-derived Babesia bovis exoantigen using a two-site enzyme immunoassay.

作者信息

Montealegre F, Montenegro-James S, Kakoma I, Ristic M

机构信息

Department of Veterinary Pathobiology, College of Veterinary Medicine, University of Illinois, Urbana 61801.

出版信息

J Clin Microbiol. 1987 Sep;25(9):1648-52. doi: 10.1128/jcm.25.9.1648-1652.1987.

Abstract

Soluble exoantigens in the supernatants of Babesia bovis cultures have been shown to be efficient immunogens against bovine babesiosis. We used a two-site enzyme immunoassay to monitor the release of these antigens during in vitro cultivation. Bovine immunoglobulin G was isolated from serum of an adult cow previously immunized with culture-derived B. bovis exoantigens and challenged via needle with virulent parasites. The specific immunoglobulin G was used as a capture antibody and as an enzyme-conjugated recognizing antibody. The optimal protein concentration of capture antibody was 10 micrograms/ml. The 24-h cultures showed the greatest antigen concentration. The test was sensitive for detection of differences in species-specific antigenic activity among B. bovis isolates, for determining loss of antigenicity during storage and formalinization, and for monitoring the kinetics of exoantigen release during in vitro cultivation. Antigens cross-reactive with the other major Babesia species of cattle, Babesia bigemina, were also detected with this assay. The high specificity, sensitivity, and reproducibility of this technique should facilitate detection and quantitation of Babesia antigens during purification and in standardization of candidate immunogens.

摘要

牛巴贝斯虫培养上清液中的可溶性外抗原已被证明是抗牛巴贝斯虫病的有效免疫原。我们使用双位点酶免疫测定法监测体外培养过程中这些抗原的释放。从先前用培养来源的牛巴贝斯虫外抗原免疫并经毒力寄生虫针刺攻击的成年母牛血清中分离出牛免疫球蛋白G。特异性免疫球蛋白G用作捕获抗体和酶联识别抗体。捕获抗体的最佳蛋白浓度为10微克/毫升。24小时培养物显示出最高的抗原浓度。该试验对于检测牛巴贝斯虫分离株之间物种特异性抗原活性的差异、确定储存和福尔马林固定过程中抗原性的丧失以及监测体外培养过程中外抗原释放的动力学很敏感。用该测定法还检测到与牛的其他主要巴贝斯虫物种双芽巴贝斯虫交叉反应的抗原。该技术的高特异性、敏感性和可重复性应有助于在候选免疫原的纯化和标准化过程中检测和定量巴贝斯虫抗原。

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