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用于通过逆转录-聚合酶链反应检测李痘病毒的不同RNA提取方法的比较

Comparison of different methods of RNA isolation for plum pox virus detection by reverse transcription-polymerase chain reaction.

作者信息

Faggioli F, Pasquini G, Barba M

机构信息

Istituto Sperimentale per la Patologia Vegetale, Rome, Italy.

出版信息

Acta Virol. 1998 Sep;42(4):219-21.

PMID:10073221
Abstract

The diagnosis of plum pox virus (PPV) is still considered one of the most important aspects of the "sharka" problem. In fact, different studies demonstrated an uneven distribution of the virus in infected trees due to a high variability in virus concentration. These aspects complicate the PPV diagnosis. To date, biological, serological and molecular assays have been successively developed in order to obtain sensitive and efficient PPV detection techniques. In particular, the polymerase chain reaction (PCR) technique seems to be promising and can be considered the most sensitive and reliable one. Preparation of viral RNA is still a fundamental step in reverse transcription-PCR (RT-PCR) technique, especially when applied to large scale testing, i.e., for certification purposes. In order to find the most rapid and efficient procedure, we have compared three different procedures of extraction of viral RNA to be processed RT-PCR. Their common characteristics is their capacity to extract the RNA from a small amount of plant tissue without organic solvents in the extraction fluid. The procedures were as follows: an immuno-capture (IC) method using a specific antiserum, a silica-capture (SC) method using a non-specific matrix, and a simple and rapid RNA extraction (RE) method. They all were followed by one-tube RT-PCR. The obtained results show that all the three techniques allowed a successful amplification and detection of PPV in tested samples except the SC-PCR method which proved less effective. In fact, the IC-PCR and RE-PCR methods amplified and detected PPV in all isolates tested, while the SC-PCR method was able to reveal the presence of the virus in apricot and infected control samples only.

摘要

李痘病毒(PPV)的诊断仍被视为“李痘病”问题最重要的方面之一。事实上,不同研究表明,由于病毒浓度变化很大,该病毒在受感染树木中的分布并不均匀。这些情况使PPV的诊断变得复杂。迄今为止,人们先后开发了生物学、血清学和分子检测方法,以获得灵敏且高效的PPV检测技术。特别是,聚合酶链反应(PCR)技术似乎很有前景,可被认为是最灵敏可靠的技术。病毒RNA的制备仍是逆转录PCR(RT-PCR)技术的一个基本步骤,尤其是在应用于大规模检测(即用于认证目的)时。为了找到最快速高效的方法,我们比较了三种不同的用于RT-PCR的病毒RNA提取方法。它们的共同特点是能够从少量植物组织中提取RNA,且提取液中不含有机溶剂。这些方法如下:使用特异性抗血清的免疫捕获(IC)法、使用非特异性基质的硅胶捕获(SC)法以及一种简单快速的RNA提取(RE)法。之后都进行单管RT-PCR。所得结果表明,除SC-PCR方法效果较差外,所有这三种技术都能成功扩增并检测出测试样品中的PPV。实际上,IC-PCR和RE-PCR方法在所有测试分离株中都扩增并检测出了PPV,而SC-PCR方法仅能在杏树和受感染对照样品中检测到病毒的存在。

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