Arrigo S, Beemon K
Department of Biology, Johns Hopkins University, Baltimore, Maryland 21218.
Mol Cell Biol. 1988 Nov;8(11):4858-67. doi: 10.1128/mcb.8.11.4858-4867.1988.
Only a fraction of retroviral primary transcripts are spliced to subgenomic mRNAs; the unspliced transcripts are transported to the cytoplasm for packaging into virions and for translation of the gag and pol genes. We identified cis-acting sequences within the gag gene of Rous sarcoma virus (RSV) which negatively regulate splicing in vivo. Mutations were generated downstream of the splice donor (base 397) in the intron of a proviral clone of RSV. Deletion of bases 708 to 800 or 874 to 987 resulted in a large increase in the level of spliced RSV RNA relative to unspliced RSV RNA. This negative regulator of splicing (nrs) also inhibited splicing of a heterologous splice donor and acceptor pair when inserted into the intron. The nrs element did not affect the level of spliced RNA by increasing the rate of transport of the unspliced RNA to the cytoplasm but interfered more directly with splicing. To investigate the possible role of gag proteins in splicing, we studied constructs carrying frameshift mutations in the gag gene. While these mutations, which caused premature termination of gag translation, did not affect the level of spliced RSV RNA, they resulted in a large decrease in the accumulation of unspliced RNA in the cytoplasm.
只有一小部分逆转录病毒初级转录本会被剪接成亚基因组mRNA;未剪接的转录本会被转运到细胞质中,用于包装进病毒粒子以及翻译gag和pol基因。我们在劳氏肉瘤病毒(RSV)的gag基因中鉴定出了在体内对剪接起负调控作用的顺式作用序列。在RSV前病毒克隆的内含子中,于剪接供体(第397位碱基)下游产生了突变。缺失第708至800位碱基或第874至987位碱基会导致剪接的RSV RNA水平相对于未剪接的RSV RNA大幅增加。这种剪接负调控因子(nrs)插入内含子时,也会抑制异源剪接供体和受体对的剪接。nrs元件并非通过提高未剪接RNA向细胞质的转运速率来影响剪接RNA的水平,而是更直接地干扰剪接过程。为了研究gag蛋白在剪接中可能发挥的作用,我们研究了在gag基因中携带移码突变的构建体。虽然这些导致gag翻译提前终止的突变并不影响剪接的RSV RNA水平,但它们会使细胞质中未剪接RNA的积累大幅减少。