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人类异尖线虫病的诊断:重组变应原Ani s 1和Ani s 7与UniCAP 100荧光酶免疫分析的比较

Diagnosing human anisakiasis: recombinant Ani s 1 and Ani s 7 allergens versus the UniCAP 100 fluorescence enzyme immunoassay.

作者信息

Anadón A M, Rodríguez E, Gárate M T, Cuéllar C, Romarís F, Chivato T, Rodero M, González-Díaz H, Ubeira F M

机构信息

Laboratorio de Parasitología, Universidad de Santiago de Compostela, 15782 Santiago de Compostela, Spain.

出版信息

Clin Vaccine Immunol. 2010 Apr;17(4):496-502. doi: 10.1128/CVI.00443-09. Epub 2010 Jan 27.

Abstract

Commercially available serological methods for serodiagnosis of human anisakiasis either are poorly specific or do not include some of the most relevant Anisakis allergens. The use of selected recombinant allergens may improve serodiagnosis. To compare the diagnostic and clinical values of enzyme-linked immunosorbent assay (ELISA) methods based on Ani s 1 and Ani s 7 recombinant allergens and of the UniCAP 100 fluorescence enzyme immunoassay (CAP FEIA) system, we tested sera from 495 allergic and 25 non-food-related allergic patients. The decay in specific IgE antibodies in serum was also investigated in 15 positive patients over a period of 6 to 38 months. Considering sera that tested positive by either Ani s 1 or Ani s 7 ELISA, the CAP FEIA classified 25% of sera as falsely positive, mainly in the group of patients with the lowest levels of anti-Anisakis IgE antibodies, and 1.28% of positive sera as falsely negative. Considering allergens individually, the overall sensitivities of Ani s 7 ELISA and Ani s 1 ELISA were 94% and 61%, respectively. The results also showed that anti-Anisakis IgE antibodies can be detected in serum for longer with Ani s 1 ELISA than with Ani s 7 ELISA and CAP FEIA (P < 0.01). Our findings suggest that ELISA methods with Ani s 7 and Ani s 1 allergens as targets of IgE antibodies are currently the best option for serodiagnosis of human anisakiasis, combining specificity and sensitivity. The different persistence of anti-Ani s 1 and anti-Ani s 7 antibodies in serum may help clinicians to distinguish between recent and old Anisakis infections.

摘要

用于人类异尖线虫病血清诊断的市售血清学方法,要么特异性较差,要么未涵盖一些最相关的异尖线虫过敏原。使用选定的重组过敏原可能会改善血清诊断。为比较基于Ani s 1和Ani s 7重组过敏原的酶联免疫吸附测定(ELISA)方法与UniCAP 100荧光酶免疫测定(CAP FEIA)系统的诊断和临床价值,我们检测了495名过敏患者和25名非食物相关过敏患者的血清。还对15名阳性患者在6至38个月的时间内血清中特异性IgE抗体的衰减情况进行了研究。考虑到通过Ani s 1或Ani s 7 ELISA检测呈阳性的血清,CAP FEIA将25%的血清分类为假阳性,主要在抗异尖线虫IgE抗体水平最低的患者组中,以及将1.28%的阳性血清分类为假阴性。单独考虑过敏原时,Ani s 7 ELISA和Ani s 1 ELISA的总体敏感性分别为94%和61%。结果还表明,与Ani s 7 ELISA和CAP FEIA相比,使用Ani s 1 ELISA在血清中检测抗异尖线虫IgE抗体的时间更长(P < 0.01)。我们的研究结果表明,以Ani s 7和Ani s 1过敏原作为IgE抗体靶点的ELISA方法,结合了特异性和敏感性,是目前人类异尖线虫病血清诊断的最佳选择。血清中抗Ani s 1和抗Ani s 7抗体的不同持续时间可能有助于临床医生区分近期和既往的异尖线虫感染。

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