利用免疫印迹血清学试验诊断巴贝斯虫病

R. Ryan, P. Krause, J. Radolf, K. Freeman, A. Spielman, Ronald Lenz, Andrew E. Levin
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引用次数: 28

摘要

虽然目前的间接免疫荧光法(IFA)诊断人类巴贝斯虫病的抗体测试是敏感和特异性的,但免疫印迹抗体测试可能更容易标准化和执行。因此,我们的目的是确定使用巴贝斯虫微全细胞裂解液作为抗原的诊断急性人类巴贝斯虫病的免疫印迹抗体试验的有效性并制定解释标准。我们比较了24名出现巴贝斯虫病症状并有实验室证据的人类受试者,28名患有莱姆病的受试者,12名患有人粒细胞埃利希体病的受试者,以及51名没有这些疾病史且血清对b虫无反应的受试者的血清对b虫免疫印迹检测的反应性。在IFA试验中发现微量抗原。免疫印迹条中浸渍了从大肠杆菌的GI菌株中提取的蛋白质,这些蛋白质在丙烯酰胺十二烷基硫酸钠凝胶中电泳,然后电印迹到硝化纤维素膜上。所有经历过巴贝斯虫病的受试者的血清在IFA中对微小贝氏杆菌抗原和对微小贝氏杆菌特异性的9个免疫印迹蛋白带中的至少一个发生反应。相比之下,那些似乎没有经历过这种感染的人的血清在IFA中没有对微螺旋体抗原产生反应(相比之下,免疫印迹试验中有4%)。当两个反应带被认为是决定性的,免疫印迹试验敏感性为96%,特异性为99%,预测阳性和预测阴性分别为96%和99%。我们的微孢子虫免疫印迹方法有望成为急性巴贝斯虫病常规临床诊断的一种敏感、特异和可重复的检测方法。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Diagnosis of Babesiosis Using an Immunoblot Serologic Test
ABSTRACT Although the current indirect immunofluorescent assay (IFA) diagnostic antibody test for human babesiosis is sensitive and specific, an immunoblot antibody test may be easier to standardize and to perform. Our objective, therefore, was to determine the efficacy of and develop interpretive criteria for an immunoblot antibody test for diagnosing acute human babesiosis using a Babesia microtiwhole-cell lysate as the antigen. We compared the reactivity of sera to a B. microti immunoblot assay in 24 human subjects experiencing symptoms and expressing laboratory evidence of babesiosis, 28 subjects who experienced Lyme disease, 12 subjects who experienced human granulocytic ehrlichiosis, and 51 subjects who reported no history of any of these diseases and whose sera did not react againstB. microti antigen in an IFA test. Immunoblot strips were impregnated with proteins derived from the GI strain of B. microti that had been electrophoresed in an acrylamide sodium dodecyl sulfate gel, followed by electroblotting onto nitrocellulose membranes. The sera of all subjects who experienced babesiosis reacted against the B. microti antigen in the IFA and against at least one of nine immunoblot protein bands specific to B. microti. In contrast, none of the sera from people who appeared not to have experienced this infection reacted against the B. microti antigen in the IFA (compared to 4% in the immunoblot assay). When two reactive bands were considered as definitive, immunoblot test sensitivity was 96%, while specificity was 99% and predictive positivity and predictive negativity were 96 and 99%, respectively. Our B. microti immunoblot procedure shows promise as a sensitive, specific, and reproducible assay for routine clinical diagnosis of acute babesiosis.
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