Hayes R J, Buck K W
Department of Biology, Imperial College of Science, Technology and Medicine, London, U.K.
J Gen Virol. 1990 Nov;71 ( Pt 11):2503-8. doi: 10.1099/0022-1317-71-11-2503.
Full-length cDNA to RNA 1, RNA 2 and RNA 3 of cucumber mosaic virus strain Q (CMV-Q) was amplified using the polymerase chain reaction (PCR). The first-strand primer contained a BamHI site and sequences complementary to the 3' terminus of the RNA. The second-strand primers contained a BamHI site, a T7 promoter and sequences corresponding to the 5' terminus of each RNA. After cleavage with BamHI, the PCR products were cloned into the BamHI site of the vector pEMBL9(+). Five clones of each RNA were selected and RNA transcripts were synthesized in vitro from each clone using T7 RNA polymerase. The constructs were designed to allow transcription to initiate precisely at the 5' terminus of each RNA. All the transcripts were found to be infectious when inoculated onto Nicotiana tabacum cv. Samsun plants in sets of three, corresponding to RNA 1, RNA 2 and RNA 3. Of the transcript sets, four induced symptoms indistinguishable from symptoms induced by CMV-Q RNAs. However a fifth transcript set induced much more severe symptoms. Plasmids were also constructed to allow synthesis of transcripts with one or two additional G residues at the 5' terminus of each RNA. Although the yields of such transcripts synthesized in vitro with T7 RNA polymerase were higher, their infectivity was lower than that of those with no additional residues at their 5' termini.
利用聚合酶链反应(PCR)扩增黄瓜花叶病毒Q株(CMV-Q)RNA 1、RNA 2和RNA 3的全长cDNA。第一链引物包含一个BamHI位点以及与RNA 3'末端互补的序列。第二链引物包含一个BamHI位点、一个T7启动子以及与各RNA 5'末端对应的序列。用BamHI切割后,将PCR产物克隆到载体pEMBL9(+)的BamHI位点。每个RNA选取5个克隆,并使用T7 RNA聚合酶从每个克隆体外合成RNA转录本。构建体的设计使得转录能在各RNA的5'末端精确起始。将所有转录本以三个一组接种到烟草品种三生烟植株上时,发现它们都具有感染性,这三个一组分别对应RNA 1、RNA 2和RNA 3。在这些转录本组中,有四组诱导出的症状与CMV-Q RNA诱导的症状无法区分。然而,第五个转录本组诱导出的症状要严重得多。还构建了质粒,以允许在各RNA的5'末端合成带有一个或两个额外G残基的转录本。尽管用T7 RNA聚合酶体外合成的这类转录本产量较高,但其感染性低于5'末端没有额外残基的转录本。
