Scott J M, Imperiale M J
Department of Microbiology and Immunology, University of Michigan Medical School, Ann Arbor 48109-0620, USA.
Mol Cell Biol. 1997 Apr;17(4):2127-35. doi: 10.1128/MCB.17.4.2127.
The presence of two polyadenylation signals in the primary transcript of the human immunodeficiency virus type 1 (HIV-1) provirus leads to a requirement for regulation of 3'-end processing. To ensure that viral genome replication and gene expression occur, polyadenylation must occur at the poly(A) site transcribed from the 3' long terminal repeat (LTR) but not the 5' LTR. Models that have been proposed to explain this regulation include (i) inhibition of the 5' site as a result of proximity to the promoter and (ii) enhancement of the 3' site by U3 sequences that are transcribed upstream of only the 3' poly(A) site. In previous studies designed to investigate these models, a reduction in the levels of steady-state RNA was observed when the HIV-1 poly(A) site was placed within 500 nucleotides of the cap site. Although these findings were interpreted to be the result of promoter proximity effects on 3'-end processing, in vitro studies demonstrated that the HIV-1 poly(A) site was equally functional in promoter-proximal and promoter-distal positions. These results led to the hypothesis that, in vivo, the poly(A) site is fully active at this close distance but the short transcripts produced are highly unstable in the nucleus and undergo rapid degradation, precluding their appearance as abundant mRNAs in the steady-state pool. To investigate the biogenesis of these short RNAs in vivo, experiments were performed to examine directly the nuclear processing rates of the HIV-1 poly(A) site in intact cells. By using recombinant adenoviruses as expression vectors, it is now demonstrated conclusively that the HIV-1 poly(A) site is indeed processed at equivalent levels independent of its distance from the promoter. Although transcripts containing the promoter-proximal poly(A) site are processed efficiently, most undergo degradation in the nucleus instead of nucleocytoplasmic transport.
人类免疫缺陷病毒1型(HIV-1)前病毒的初级转录本中存在两个聚腺苷酸化信号,这导致了对3'端加工调控的需求。为确保病毒基因组复制和基因表达的发生,聚腺苷酸化必须发生在从3'长末端重复序列(LTR)转录的聚(A)位点,而不是5' LTR。已提出的解释这种调控的模型包括:(i)由于靠近启动子而抑制5'位点;(ii)通过仅在3'聚(A)位点上游转录的U3序列增强3'位点。在先前旨在研究这些模型的研究中,当HIV-1聚(A)位点位于帽位点500个核苷酸范围内时,观察到稳态RNA水平降低。尽管这些发现被解释为启动子接近效应影响3'端加工的结果,但体外研究表明,HIV-1聚(A)位点在启动子近端和远端位置具有同等功能。这些结果导致了这样一种假设,即在体内,聚(A)位点在这个近距离时是完全活跃的,但产生的短转录本在细胞核中高度不稳定并迅速降解,从而阻止它们在稳态池中以丰富的mRNA形式出现。为了研究这些短RNA在体内的生物合成,进行了实验以直接检查完整细胞中HIV-1聚(A)位点的核加工速率。通过使用重组腺病毒作为表达载体,现在已确凿证明,HIV-1聚(A)位点确实以等效水平进行加工,而与它距启动子的距离无关。尽管含有启动子近端聚(A)位点的转录本被有效加工,但大多数在细胞核中经历降解,而不是进行核质运输。