The coat protein gene of isolates of citrus tristeza virus (CTV) from 20 citrus-producing regions around the world was amplified by RT-PCR, TA cloned, and characterized by SSCP. Haplotypes that produced different patterns within each geographic region were sequenced and a database of 153 accessions of CTV was assembled. Phylogenetic analysis revealed the existence of seven well-defined clusters (Coefficient of differentiation 0.78). An asymmetric PCR-ELISA typing (APET) assay was developed in the frame of this clustering pattern using a set of eight hybridisation probes. The membership of any unknown haplotype is determined by comparing its pattern of reaction against the whole set of probes and not, as previously done in hybridisation assays, in an all-or-nothing basis. Interpretation of the results is objective and done through a visual basic application that compares the rates of hydrolysis of the ELISA substrate of an assayed isolate to a matrix of rates of hydrolysis obtained from standard haplotypes. This assay was validated and showed a better ability to resolve haplotypes than other assays to which it was compared experimentally. It may be automated to the same extent as any ELISA.

译文

:通过RT-PCR扩增了来自全球20个柑橘产区的柑橘变形杆菌病毒(CTV)分离株的外壳蛋白基因,TA克隆并通过SSCP进行了鉴定。对在每个地理区域内产生不同模式的单倍体进行测序,并收集了153份CTV的数据库。系统发育分析显示存在七个明确定义的簇(分化系数0.78)。使用一组八种杂交探针,在这种聚类模式的框架内开发了一种不对称PCR-ELISA分型(APET)测定法。通过将其反应模式与整套探针进行比较来确定任何未知单倍型的成员,而不是像以前在杂交测定中所做的那样,不是全有还是全无。结果的解释是客观的,并且是通过视觉基础应用程序完成的,该应用程序将测定的分离物的ELISA底物的水解速率与从标准单倍型获得的水解速率矩阵进行比较。该试验已经过验证,与其他试验进行了比较,它显示出更好的分辨单倍型的能力。它可以自动化到与任何ELISA相同的程度。

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