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Comparison of the immunofluorescence assay with RT-PCR and nested PCR in the diagnosis of canine distemper.

机译:免疫荧光测定与RT-PCR和巢式PCR在犬瘟热的诊断中的比较。

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摘要

Two pairs of primers were prepared, both localized within the sequences of the nucleoprotein gene (NP) of canine distemper virus (CDV). A number of experiments were done to optimize the conditions of RT-PCR and nested PCR methods. The nucleic acids of the Onderstepoort, Rockborn, Snyder Hill and Lederle strains of CDV could be detected with these primers. However, they did not react with the sequences of the Edmonston strain of the measles virus. The detection limit for RT-PCR was 10 TCID50 and for nested PCR 0.1 TCID50 of CDV. The RT-PCR was able to demonstrate the nucleic acid of CDV in the blood of all seven puppies vaccinated with a modified live virus. Blood samples of 23 dogs clinically suspected of distemper were examined by RT-PCR combined with nested PCR, and the results were compared with the detection of the CDV antigen in the smears from the mucous membranes by the direct immunofluorescence (IF) test. Of the 23 dogs, 12 were positive in nested PCR, six in the IF assay, and only two in single RT-PCR. It is concluded that nested PCR seems to be the most sensitive method for ante-mortem diagnosis of canine distemper, especially in its subacute or chronic forms.
机译:制备两对引物,均在犬瘟热病毒(CDV)的核蛋白基因(NP)的序列内局部化。进行了许多实验以优化RT-PCR和嵌套PCR方法的条件。可以用这些引物检测onderstepoort,Roceborn,斯奈德山和CDV的Lederle菌株的核酸。然而,它们没有与麻疹病毒的edmonston菌株的序列反应。 RT-PCR的检测限为10个TCID50,并且用于CDV的嵌套PCR 0.1 TCID50。 RT-PCR能够用修饰的活病毒接种疫苗的所有七只小狗的血液中的CDV核酸。通过RT-PCR与巢式PCR相结合检查23只狗的血液样品,并将结果与​​嵌套的PCR联合,并将结果与​​通过直接免疫荧光(IF)试验检测来自粘膜的涂片中的CDV抗原。在23只狗中,12只嵌套PCR阳性,IF测定中的六个,在单个RT-PCR中只有两个。结论是,嵌套的PCR似乎是犬瘟热的诊断最敏感的方法,特别是其亚急性或慢性形式。

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