A Comparison of Different PCR-Based Methods for the Detection of African Horsesickness Virus

C. Bremer
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引用次数: 1

Abstract

Detection of African horsesickness virus (AHSV) by three different reverse transcription polymerase chain reaction (RT-PCR) based methods were compared. Primers were complementary to sequences contained in the gene encoding non-structural protein 2 of AHSV serotype 3. All three assays were group-specific for AHSV and detected all nine serotypes but not related orbiviruses. A dilution range was made of titrated chicken embryo-related cells infected with AHSV serotype 3 and, after isolating RNA from each diluted sample they were tested using the three different assays. RNA representing 0.2, 2 and 20 plaque forming units of AHSV could be detected by hemi-nested RT-PCR, PCR- enzyme-linked immunosorbent assay (PCR-ELISA) and RT-PCR respectively. In twelve samples from African horsesickness suspect field cases hemi-nested RT-PCR, intra-cerebral injection of mice and virus isolation from cell culture detected AHSV in 83%, 58% and 25% of samples respectively.
非洲马蹄疫病毒不同pcr检测方法的比较
比较了三种基于逆转录聚合酶链反应(RT-PCR)的检测方法对非洲马蹄疫病毒(AHSV)的检测效果。引物与AHSV血清3型非结构蛋白2编码基因序列互补。这三种检测方法均对AHSV具有群体特异性,并检测到所有9种血清型,但未检测到相关的轨道病毒。稀释范围由感染3型AHSV血清型的经滴定的鸡胚相关细胞组成,并在从每个稀释样品中分离RNA后,使用三种不同的检测方法进行测试。半巢式RT-PCR、PCR-酶联免疫吸附法(PCR- elisa)和RT-PCR分别检测到AHSV斑块形成单位为0.2、2和20的RNA。在12份非洲马蹄疫疑似病例样本中,半巢式RT-PCR、小鼠脑内注射和细胞培养病毒分离分别检出83%、58%和25%的AHSV。
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