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首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Evaluation of a Microplate Latex Agglutination Method (Verotox-F Assay) for Detecting and Characterizing Verotoxins (Shiga Toxins) in Escherichia coli
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Evaluation of a Microplate Latex Agglutination Method (Verotox-F Assay) for Detecting and Characterizing Verotoxins (Shiga Toxins) in Escherichia coli

机译:微孔板乳胶凝集法(Verotox-F测定)用于检测和鉴定大肠杆菌中毒素(志贺毒素)的评估

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The performance of a commercial microplate latex agglutination assay, the Verotox-F assay, was compared with that of the Vero cell assay for the detection and characterization of Escherichia coli verocytotoxins (VTs). Culture filtrates of 68 VT-positive E. coli strains (65 human isolates [33 of serotype O157:H7/H−, 32 of non-O157 serotypes] and 3 reference strains) and 104 VT-negative strains (100 human isolates and 4 reference strains) were investigated. The toxin phenotypes and genotypes of the 68 VT-positive isolates were VT1 only (18 strains), VT2 and/or VT2c (33 strains), and VT1 plus VT2 (17 strains). The Verotox-F assay involved incubation of serial dilutions of culture filtrates with equal volumes of latex particles sensitized with anti-VT1 antibody or anti-VT2 antibody in 96-well microtiter plates with appropriate controls and examination for latex agglutination after 20 to 24 h. Compared to the results of the Vero cell assay, the Verotox-F assay was 100% sensitive and 100% specific for the detection of VTs in culture filtrates and correctly identified the toxin types of all 68 VT producers. By checkerboard titration with purified toxins, the sensitivity of the Verotox-F assay was found to be 14 pg (0.7 ng/ml) for VT1, 12 pg (0.6 ng/ml) for VT2, and 350 pg (17.5 ng/ml) for VT2c; this sensitivity is comparable to that of the bioassay. The anti-VT2 latex reagent detected both VT2 and VT2c and did not cross-react with VT1. The anti-VT1 reagent showed a low-level cross-reaction with VT2c only at levels (≥4.5 μg/ml) that were about 1,000-fold higher than those found in culture filtrates. We conclude that the Verotox-F assay is highly sensitive and specific for the detection and characterization of VTs in culture filtrates of human E. coli isolates. The test is rapid, reliable, and easy to perform; its results are easy to interpret; and it should allow testing for VT to become more widely performed.
机译:比较了商用微孔板乳胶凝集测定法(Verotox-F测定法)与Vero细胞测定法的性能,以检测和鉴定大肠埃希氏菌毒素(VTs)。 68种VT阳性大肠杆菌菌株(65种人类分离株[33种O157:H7 / H-血清型,32种非O157血清型]和3种参考菌株)的培养液和104种VT阴性菌株(100种人类分离株和4种参考菌株)。 68个VT阳性分离株的毒素表型和基因型分别为VT1(18株),VT2和/或VT2c(33株)以及VT1加VT2(17株)。 Verotox-F分析包括将培养滤液的连续稀释液与等体积的用抗VT1抗体或抗VT2抗体敏化的乳胶颗粒在适当控制下的96孔微量滴定板中孵育,并在20至24小时后检查乳胶凝集情况。与Vero细胞分析的结果相比,Verotox-F分析对培养滤液中VT的检测具有100%的敏感性和100%的特异性,并正确鉴定了所有68个VT生产者的毒素类型。通过用纯化毒素进行棋盘滴定,发现Verotox-F分析的灵敏度对于VT1为14 pg(0.7 ng / ml),对于VT2为12 pg(0.6 ng / ml),而对于VT2为350 pg(17.5 ng / ml)对于VT2c;该灵敏度与生物测定法相当。抗VT2乳胶试剂同时检测到VT2和VT2c,并且未与VT1交叉反应。抗VT1试剂仅在水平(≥4.5μg/ ml)时才与VT2c发生低水平的交叉反应,该水平比培养物滤液中的水平高约1,000倍。我们得出的结论是,Verotox-F分析对人大肠杆菌分离株培养滤液中的VT的检测和表征具有很高的敏感性和特异性。该测试快速,可靠且易于执行;其结果易于解释;并且应该使VT的测试变得更加广泛。

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