首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Purification of a Brucella canis cell wall antigen by using immunosorbent columns and use of the antigen in enzyme-linked immunosorbent assay for specific diagnosis of canine brucellosis.
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Purification of a Brucella canis cell wall antigen by using immunosorbent columns and use of the antigen in enzyme-linked immunosorbent assay for specific diagnosis of canine brucellosis.

机译:通过使用免疫吸附柱纯化犬布鲁氏菌细胞壁抗原并将其用于酶联免疫吸附测定中以特异性诊断犬布鲁氏菌病。

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摘要

A cell wall antigen of Brucella canis was purified by immunosorbent columns. The antigen contained two proteins of 30 and 28 kilodaltons and a polysaccharide exhibiting a 12-kilodalton band upon 12.5% sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Antibody to the purified antigen, which specifically reacted with the polysaccharide, was used as the first coating antibody in an enzyme-linked immunosorbent assay (ELISA) for serological diagnosis of canine brucellosis. Dogs inoculated orally with live B. canis were positive and dogs from B. canis-free colonies were negative in the ELISA. Of 199 dogs from a brucellosis-contaminated area, 116 with negative titers in the tube agglutination test (TAT), using heat-inactivated whole B. canis cells as the antigen, were also negative in the ELISA. Seventy-eight of the dogs with questionable titers in the TAT were divided into two groups: 20 dogs that were positive in the ELISA and 58 that were negative. Of five dogs with positive titers in the TAT, three were positive in the ELISA and the gel immunodiffusion test (GD) with crude B. canis extract as the antigen and were also culture positive for B. canis. One dog was positive in the ELISA and GD but gave a negative culture result. Serum from the remaining dog, which was positive with high titer in the TAT but negative in the ELISA and in culture for B. canis, formed a spur precipitate with a homologous precipitate in the GD. These results indicate that the ELISA is a specific serological test for B. canis infection in dogs.
机译:通过免疫吸附柱纯化犬布鲁氏菌的细胞壁抗原。该抗原包含两种分别为30和28千道尔顿的蛋白质,以及一种在12.5%的十二烷基硫酸钠-聚丙烯酰胺凝胶电泳时显示12千达尔顿带的多糖。与多糖特异性反应的纯化抗原的抗体被用作酶联免疫吸附测定(ELISA)中的第一道包被抗体,用于血清学诊断犬布鲁氏菌病。 ELISA中,口服活犬双歧杆菌的狗为阳性,无犬双歧杆菌菌落的狗为阴性。在来自布鲁氏菌病污染地区的199只狗中,使用热灭活的整个犬双歧杆菌细胞作为抗原的试管凝集试验(TAT)中滴度为负的116只狗在ELISA中也呈阴性。将TAT中效价可疑的78只狗分为两组:20只在ELISA中呈阳性的狗和58只呈阴性的狗。在TAT滴度为阳性的5只狗中,有3只在ELISA和以粗制犬双歧杆菌提取物为抗原的凝胶免疫扩散试验(GD)中呈阳性,并且对犬双歧杆菌也呈阳性。一只狗的ELISA和GD呈阳性,但培养结果为阴性。来自剩下的狗的血清在TAT中呈高滴度呈阳性,而在ELISA和犬双歧杆菌培养中呈阴性,形成了马刺沉淀,在GD中形成了同源沉淀。这些结果表明,ELISA是针对狗的犬双歧杆菌感染的特异性血清学测试。

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