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用于检测马流感病毒的病毒分离、抗原检测和核酸扩增的敏感性比较。

Comparison of sensitivities of virus isolation, antigen detection, and nucleic acid amplification for detection of equine influenza virus.

作者信息

Quinlivan Michelle, Cullinane Ann, Nelly Maura, Van Maanen Kees, Heldens Jacco, Arkins Sean

机构信息

Virology Unit, Irish Equine Centre, Johnstown, Naas, County Kildare, Ireland.

出版信息

J Clin Microbiol. 2004 Feb;42(2):759-63. doi: 10.1128/JCM.42.2.759-763.2004.

Abstract

Four seronegative foals aged 6 to 7 months were exposed to an aerosol of influenza strain A/Equi/2/Kildare/89 at 10(6) 50% egg infective doses (EID(50))/ml. Nasopharyngeal swabs were collected for 10 consecutive days after challenge. Virus isolation was performed in embryonated eggs, and the EID(50) was determined for all positive samples. The 50% tissue culture infective dose was determined using Madin-Darby canine kidney (MDCK) cells. Samples were also tested by an in vitro enzyme immunoassay test, Directigen Flu A, and by reverse transcription-PCR (RT-PCR) using nested primers from the nucleoprotein gene and a single set of primers from the matrix gene. RT-PCR using the matrix primers and virus isolation in embryonated eggs proved to be the most sensitive methods for the detection of virus. The Directigen Flu A test was the least sensitive method. The inclusion of 2% fetal calf serum in the viral transport medium inhibited the growth of virus from undiluted samples in MDCK cells but was essential for the maintenance of the virus titer in samples subjected to repeated freeze-thaw cycles.

摘要

4匹6至7月龄的血清学阴性马驹暴露于含有A/Equi/2/Kildare/89流感毒株气溶胶中,浓度为10(6) 50%鸡胚感染剂量(EID(50))/毫升。攻毒后连续10天采集鼻咽拭子。在鸡胚中进行病毒分离,并对所有阳性样本测定EID(50)。使用犬肾传代细胞(MDCK)测定50%组织培养感染剂量。样本还通过体外酶免疫测定试验Directigen Flu A以及使用核蛋白基因的巢式引物和基质基因的单套引物进行逆转录聚合酶链反应(RT-PCR)检测。使用基质引物的RT-PCR和在鸡胚中进行病毒分离被证明是检测病毒最敏感的方法。Directigen Flu A试验是最不敏感的方法。病毒运输培养基中加入2%胎牛血清可抑制未稀释样本中的病毒在MDCK细胞中的生长,但对于经反复冻融循环的样本维持病毒滴度至关重要。

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