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用于班氏丝虫病IgG-ELISA诊断的犬恶丝虫成虫的大小和电荷抗原

Size and charge antigens of Dirofilaria immitis adult worm for IgG-ELISA diagnosis of bancroftian filariasis.

作者信息

Riyong Doungrat, Waikagul Jitra, Panasoponkul Chotechuang, Choochote Wej, Ito Akira, Dekumyoy Paron

机构信息

Department of Parasitology, Faculty of Medicine, Chiang Mai University, Chiang Mai.

出版信息

Southeast Asian J Trop Med Public Health. 2010 Mar;41(2):285-97.

Abstract

We used Dirofilaria immitis adult worm antigens to develop an IgG-ELISA, then used this to evaluate 30 serum samples of patients with proven Wuchereria bancrofti infection, 131 samples of patients with other parasitic diseases and 30 serum samples of healthy controls. The D. immitis antigen was prepared using two methods: Sephacryl S-200 chromatography and iso-electric focusing with a Rotofor cell. This was done to determine the best method for diagnosing W. bancrofti filariasis. Before fractionation, crude male D. immitis antigen yielded 100% sensitivity and 60.8% specificity, and crude female antigen yielded 80% sensitivity and 52.8% specificity, respectively, to detect W. bancrofti infection. After gel filtration chromatography, the male D. immitis antigen, called MP1, yielded 100% sensitivity and 95% specificity, and female D. immitis antigen, called FmP1, gave 100% sensitivity and 59.6% specificity, to detect W. bancrofti infection. Using iso-electric-focusing, both male and female crude D. immitis antigens (Iso-MF and Iso-FmF, respectively) were separated mechanically into 20 iso-fractions (F1-F20) each. By preliminary screening with ELISA, using pooled positive and negative sera, Iso-MF10, pH 7.5, and Iso-FmF14, pH 7.6, were selected. Iso-MF10 gave 100% sensitivity and 96.9% specificity, and Iso-FmF14 gave 100% sensitivity and 64% specificity. In the study, Og4C3-ELISA, for the detection of circulating filarial antigen, was also used to analyze these serum samples, it gave 87.6% sensitivity and 99.4% specificity to detect W. bancrofti infection. Male D. immitis antigens, MP1 and Iso-MF10, gave high sensitivity and specificity, and appear to be the best choices for use in an ELISA to diagnose bancroftian filariasis.

摘要

我们使用犬恶丝虫成虫抗原开发了一种IgG-ELISA,然后用其评估30份经证实感染班氏吴策线虫患者的血清样本、131份患有其他寄生虫病患者的样本以及30份健康对照者的血清样本。犬恶丝虫抗原采用两种方法制备:Sephacryl S-200层析法和使用Rotofor细胞进行等电聚焦法。这样做是为了确定诊断班氏吴策线虫病的最佳方法。在分级分离之前,粗制雄性犬恶丝虫抗原检测班氏吴策线虫感染的敏感性为100%,特异性为60.8%,粗制雌性抗原的敏感性为80%,特异性为52.8%。凝胶过滤层析后,名为MP1的雄性犬恶丝虫抗原检测班氏吴策线虫感染的敏感性为100%,特异性为95%,名为FmP1的雌性犬恶丝虫抗原的敏感性为100%,特异性为59.6%。使用等电聚焦法,雄性和雌性粗制犬恶丝虫抗原(分别为Iso-MF和Iso-FmF)均机械分离为20个等份(F1-F20)。通过使用混合阳性和阴性血清进行ELISA初步筛选,选择了pH 7.5的Iso-MF10和pH 7.6的Iso-FmF14。Iso-MF10的敏感性为100%,特异性为96.9%,Iso-FmF14的敏感性为100%,特异性为64%。在该研究中,用于检测循环丝虫抗原的Og4C3-ELISA也用于分析这些血清样本,其检测班氏吴策线虫感染的敏感性为87.6%,特异性为99.4%。雄性犬恶丝虫抗原MP1和Iso-MF10具有高敏感性和特异性,似乎是用于ELISA诊断班氏丝虫病的最佳选择。

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