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针对曲霉菌细胞壁抗原的特征明确的单克隆抗体可提高免疫测定的特异性和灵敏度。

Well-characterized monoclonal antibodies against cell wall antigen of Aspergillus species improve immunoassay specificity and sensitivity.

作者信息

Hao Wei, Pan Yu-Xian, Ding Yan-Qing, Xiao Sha, Yin Kai, Wang Ya-Di, Qiu Li-Wen, Zhang Qing-Lin, Woo Patrick C Y, Lau Susanna K P, Yuen Kwok-Yung, Che Xiao-Yan

机构信息

Center of Laboratory, Zhujiang Hospital, Southern Medical University, Guangzhou, China.

出版信息

Clin Vaccine Immunol. 2008 Feb;15(2):194-202. doi: 10.1128/CVI.00362-07. Epub 2007 Nov 21.

Abstract

The diagnosis of invasive aspergillosis (IA) based on the detection of Aspergillus galactomannan (GM) is complicated by the presence of cross-reactive GM epitopes in patient specimens. We have developed a novel and specific Aspergillus antigen-capture enzyme-linked immunosorbent assay (ELISA) by the selection of two well-characterized monoclonal antibodies from 17 candidate antibodies. The epitopes recognized by the monoclonal antibodies were present on the cell walls of the hyphae and the conidia of Aspergillus species, which were circulating or excreted as immunodominant antigens during the acute phase of IA established in the animal models. The detection of experimental Aspergillus-mediated antigenemia was suitably sensitive, and the sensitivity was comparable to that of a commercial GM detection ELISA kit (the Platelia Aspergillus assay). Moreover, the specificity of this assay was 100% when it was used to test 382 serum specimens and 120 urine specimens from healthy individuals. Cross-reactivity with other common opportunistic fungi, such as Penicillium and Candida species, and with purified GM protein derived from Aspergillus was not evident. Therefore, the chemical nature of the epitopes captured in this assay is most likely not associated with the GM structure, indicating that this newly developed Aspergillus antigen-capture ELISA is a promising tool for the diagnosis of IA without the risk of the false-positive results that are problematic with current GM antigen assays.

摘要

基于半乳甘露聚糖(GM)检测来诊断侵袭性曲霉病(IA)会因患者样本中存在交叉反应性GM表位而变得复杂。我们从17种候选抗体中筛选出两种特征明确的单克隆抗体,开发出了一种新型且特异的曲霉抗原捕获酶联免疫吸附测定法(ELISA)。这些单克隆抗体识别的表位存在于曲霉菌丝和分生孢子的细胞壁上,在动物模型中建立的IA急性期,它们作为免疫显性抗原循环或排泄。对实验性曲霉介导的抗原血症的检测具有足够的敏感性,其敏感性与商用GM检测ELISA试剂盒(Platelia曲霉检测法)相当。此外,当用该方法检测382份健康个体的血清样本和120份尿液样本时,其特异性为100%。与其他常见的机会性真菌,如青霉和念珠菌属,以及与源自曲霉的纯化GM蛋白均无明显交叉反应。因此,该检测法捕获的表位的化学性质很可能与GM结构无关,这表明这种新开发的曲霉抗原捕获ELISA是一种有前景的IA诊断工具,不会出现当前GM抗原检测存在问题的假阳性结果风险。

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