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首页> 外文期刊>Parasitology Research >Early detection of Fasciola gigantica infection in buffaloes by enzyme-linked immunosorbent assay and dot enzyme-linked immunosorbent assay
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Early detection of Fasciola gigantica infection in buffaloes by enzyme-linked immunosorbent assay and dot enzyme-linked immunosorbent assay

机译:酶联免疫吸附法和点酶联免疫吸附法早期检测水牛中巨大的Fasciola gigantica感染

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摘要

In an attempt to develop a suitable serological test for early detection of Fasciola gigantica infection in buffaloes, a group of proteins were isolated from the somatic antigen of the parasite by immunoaffinity chromatography. The process of isolation of the proteins has been standardized and significant level of repeatability was achieved. To test the diagnostic potentiality of the antigens, two serological tests, viz., enzyme-linked immunosorbent assay (ELISA) and dot enzyme-linked immunosorbent assay, were standardized using the sera from experimentally noninfected (group A) and infected (group B) animals. Further, the sensitivity and the specificity of the tests were evaluated employing the field sera from animals of different parasitic load viz., F. gigantica positive (group C), F. gigantica and Gastrothylax crumenifer positive (group D), F. gigantica and Gigantocotyle explanatum positive (group E), a group of sera without F. gigantica but other trematode infection (group F), only G. crumenifer positive (group G), only G. explanatum positive (group H), G. crumenifer and G. explanatum positive (group I), and PM negative (group J) collected from slaughterhouses of Bareilly (Uttar Pradesh, India) and Patna (Bihar, India). In plate ELISA, the sensitivity of the antigen and the test was 75.75% while the specificity was 97%, 95%, and 98%, respectively, against G. crumenifer, G. explanatum, and mixed infection of G. crumenifer and G. explanatum, respectively. In the case of dot ELISA the sensitivity was 86.5% and specificity was 92.3%, 94.7%, and 90%, respectively, against G. crumenifer, G. explanatum, and mixed infection of G. crumenifer and G. explanatum, respectively. The potentiality of the antigen in the diagnosis of field infection is discussed.
机译:为了开发一种合适的血清学检测方法,用于早期检测水牛中的巨大Fasciola gigantica感染,通过免疫亲和层析从寄生虫的体细胞抗原中分离出一组蛋白质。蛋白质的分离过程已经标准化,并且达到了很高的重复性水平。为了测试抗原的诊断潜力,使用来自实验未感染(A组)和感染(B组)的血清标准化了两种血清学检测,即酶联免疫吸附测定(ELISA)和点酶联免疫吸附测定。动物。此外,采用来自不同寄生负荷动物的野外血清,即巨无花果蝇阳性(C组),巨无花果蝇和十字花科阳性猪胃(D组),巨无花果和Gigantocotyle explanatum阳性(E组),血清中没有巨大的F. gigantica,但有其他吸虫感染(F组),仅G. crumenifer阳性(G组),仅G. explanatum阳性(H组),G。crumenifer和G从Bareilly(印度北方邦)和Patna(印度比哈尔)的屠宰场收集到的Explanatum阳性(I组)和PM阴性(J组)。在平板ELISA中,抗原和测试的敏感性分别为97.5%,95%和98%。 explanatum,分别。在点ELISA的情况下,针对十字花甘蓝,G。explanatum和十字花甘蓝和G. explanatum的混合感染的敏感性分别为86.5%和92.3%,94.7%和90%。讨论了抗原在野外感染诊断中的潜力。

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  • 来源
    《Parasitology Research》 |2008年第1期|141-150|共10页
  • 作者单位

    Division of Parasitology Indian Veterinary Research Institute Izatnagar 243122 Bareilly India;

    Division of Parasitology Indian Veterinary Research Institute Izatnagar 243122 Bareilly India;

    Division of Parasitology Indian Veterinary Research Institute Izatnagar 243122 Bareilly India;

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