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Molecular cloning of potato spindle tuber viroid (PSTV) cDNA synthesized by enzymatic elongation of PSTV-specific DNA primers: A general strategy for viroid cloning

机译:通过PSTV特异性DNA引物的酶促延伸合成的马铃薯纺锤块茎类病毒(PSTV)cDNA的分子克隆:类病毒克隆的一般策略

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Different cDNAs were synthesized by primer extension from the RNA of the severe strain KF 440 of potato spindle tuber viroid (PSTV) with the aid of reverse transcriptase using three PSTV-specific DNA molecules as primers. The cDNAs were made double-stranded and cloned into plasmid pBR 322. Various overlapping subgenomic DNA fragments were prepared from these clones and recombined in two different ways. In both cases a PSTV DNA copy was obtained which represented the entire PSTV RNA genome. The sequence of the DNA of one of the resulting full-length clones was identical with the original PSTV isolate, whereas the other clone showed one nucleotide change. On the basis of these results the advantages and problems of different strategies for the molecular cloning of the circular viroid RNA genome are discussed.
机译:通过使用三个PSTV特异性DNA分子作为引物,借助逆转录酶从马铃薯纺锤块茎类病毒(PSTV)的严重菌株KF 440的RNA中引物延伸合成不同的cDNA。将cDNA制成双链并克隆到质粒pBR 322中。从这些克隆中制备出各种重叠的亚基因组DNA片段,并以两种不同的方式重组。在这两种情况下,均获得了代表整个PSTV RNA基因组的PSTV DNA副本。所得全长克隆之一的DNA序列与原始PSTV分离株相同,而另一个克隆显示一个核苷酸变化。基于这些结果,讨论了环状病毒RNA基因组分子克隆的不同策略的优点和问题。

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