Carpenter C D, Simon A E
Department of Biochemistry and Molecular Biology, University of Massachusetts, Amherst 01003, USA.
Virology. 1996 Dec 15;226(2):153-60. doi: 10.1006/viro.1996.0641.
RNA viruses that do not have the stabilizing features of poly(A) tails or amino acids covalently linked to their 3' ends must develop other means for protecting or repairing their genomes from damage caused by cellular RNases. We previously found that deletions in the single-stranded tails of a satellite RNA (sat-RNA D) associated with turnip crinkle virus are repaired in vivo (C. D. Carpenter and A. E. Simon, 1996, J. Virol. 70, 478-486). We now extend this analysis to show that sat-RNA D transcripts with 3'-end deletions of 5 bases give rise to wild-type sat-RNA, while deletions of 6 to 11 bases result in sat-RNA with additional deletions to the -14 position joined to internal TCV genomic RNA (or other) sequence followed by replacement of the terminal C1-2UGC1-3 motif. In addition, we have determined that the selection of internal TCV sequence used in the repair of sat-RNA D 3' ends is not random and generation of these short TCV segments likely involves primer-mediated synthesis of abortive products facilitated by base-pairing between internal regions of TCV genomic RNA and oligoribonucleotides generated by abortive cycling from the 3' end of the TCV genome.
没有聚(A)尾巴或与3'末端共价连接的氨基酸等稳定特征的RNA病毒,必须开发其他方法来保护或修复其基因组免受细胞核糖核酸酶造成的损伤。我们之前发现,与芜菁皱缩病毒相关的卫星RNA(sat-RNA D)单链尾巴中的缺失在体内会被修复(C.D.卡彭特和A.E.西蒙,1996年,《病毒学杂志》70卷,478 - 486页)。我们现在扩展这项分析,以表明3'末端缺失5个碱基的sat-RNA D转录本会产生野生型sat-RNA,而缺失6至11个碱基则会导致sat-RNA出现额外缺失,直至 - 14位置,与内部芜菁皱缩病毒基因组RNA(或其他)序列相连,随后替换末端C1 - 2UGC1 - 3基序。此外,我们已经确定,用于修复sat-RNA D 3'末端的内部芜菁皱缩病毒序列的选择并非随机,这些短的芜菁皱缩病毒片段的产生可能涉及引物介导的流产产物合成,这是由芜菁皱缩病毒基因组RNA内部区域与从芜菁皱缩病毒基因组3'末端流产循环产生的寡核糖核苷酸之间的碱基配对所促进的。
