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首页> 外文期刊>Journal of Virological Methods >A highly sensitive heminested RT-PCR assay for the detection of citrus psorosis virus targeted to a conserved region of the genome.
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A highly sensitive heminested RT-PCR assay for the detection of citrus psorosis virus targeted to a conserved region of the genome.

机译:用于检测靶向基因组保守区域的柑橘类牛皮癣病毒的高灵敏度半定量RT-PCR分析。

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摘要

Psorosis is a widespread and damaging disease of citrus in many parts of the world. The causal agent is a multipartite virus with RNA genome present in very low concentration in infected citrus tissue. Diagnosis is made by biological indexing on indicator citrus seedlings, but it is a slow and costly procedure and therefore it is not used generally. No sensitive wide-spectrum assay for Citrus Psorosis virus (CPsV) has been reported based on RT-PCR. A highly sensitive heminested RT-PCR assay is described for the detection of CPsV. Fragments of 313 bp amplified from RNA 1 of different isolates were cloned and sequenced. Very high homology was found among six isolates from the citrus producing region of Argentina: 96.6-100% in nucleotide sequence. The consensus sequence obtained was used for the design of the primers for heminested PCR assay. It has been tested on different Argentine isolates, employing various methods for RNA extraction from infected tissue. This test is able to detect CPsV in dilutions of 10(10) of the original sample.
机译:牛皮癣在世界许多地方是一种广泛而有害的柑橘类疾病。该病原体是一种多部分病毒,其RNA基因组以极低的浓度存在于受感染的柑橘组织中。诊断是通过对指示性柑桔苗进行生物索引来进行的,但这是一个缓慢且昂贵的过程,因此通常不使用。尚无基于RT-PCR的灵敏的广谱柑橘柑橘病毒(CPsV)检测方法的报道。描述了一种用于检测CPsV的高度敏感的半胱氨酸RT-PCR测定法。从不同分离株的RNA 1扩增的313 bp片段被克隆并测序。在来自阿根廷柑桔产区的六个分离物中发现了非常高的同源性:核苷酸序列为96.6-100%。所获得的共有序列用于设计用于半定量PCR测定的引物。已使用多种从感染组织中提取RNA的方法在不同的阿根廷分离物中进行了测试。该测试能够检测原始样品10(10)的稀释液中的CPsV。

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