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首页> 外文期刊>Advances in Microbiology >Development of a Microplate Lectin-Capture RT-PCR (MLC-RT-PCR) for the Detection of Avian Infectious Bronchitis Virus
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Development of a Microplate Lectin-Capture RT-PCR (MLC-RT-PCR) for the Detection of Avian Infectious Bronchitis Virus

机译:用于检测禽传染性支气管炎病毒的微孔板凝集素捕获RT-PCR(MLC-RT-PCR)的开发

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Rapid, sensitive and specific methods are necessary to confirm the diagnosis of outbreaks of avian infectious bronchitis virus (IBV) infection. The amplification of IBV genome by reverse transcription followed by polymerase chain reaction (RT-PCR) has been one of the most used methods for the detection of this virus in clinical samples. To reduce the time and the number of steps in the molecular diagnosis of IBV, we developed a sensitive and rapid detection method based on viral capture by a lectin (Concanavalin A—Con A) in the microplate wells, followed by RT-PCR to amplify the S1 gene. The detection limit of IBV was 103 EID50/ml for the amplification of 5’part of the S1 gene, and 104 EID50/ml for the amplification of full S1 gene. This technique was specific for IBV detection, and no amplified products were detected for other avian viral pathogens (bursal infectious disease virus, avian metapneumovirus and Newcastle disease virus). The MLC-RT-PCR was as sensitive as conventional RT-PCR, and virus isolation method for the detection of IBV in tissue samples collected from experimentally infected birds. The MLC-RT-PCR technique demonstrated a great potential for the rapid and specific diagnosis of IBV.
机译:快速,灵敏和特异的方法对于确认诊断禽传染性支气管炎病毒(IBV)爆发很有必要。通过逆转录随后聚合酶链反应(RT-PCR)扩增IBV基因组已成为在临床样品中检测该病毒的最常用方法之一。为了减少IBV分子诊断的时间和步骤数,我们开发了一种灵敏,快速的检测方法,该方法基于微孔板中凝集素(伴刀豆球蛋白A-Con A)的病毒捕获,然后进行RT-PCR进行扩增S1基因。 IBV的检出限对于S1基因的5'部分扩增为103 EID50 / ml,对完整S1基因的扩增检测为104 EID50 / ml。该技术是专门针对IBV检测的,没有检测到其他禽病毒病原体(法氏囊感染性病毒,禽间质肺炎病毒和新城疫病毒)的扩增产物。 MLC-RT-PCR与常规RT-PCR一样灵敏,并且病毒分离方法可用于检测从实验感染的禽类收集的组织样本中的IBV。 MLC-RT-PCR技术证明了快速,特异性诊断IBV的巨大潜力。

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