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体外HIV-2/SIV RNA二聚化位点的鉴定揭示了与HIV-1的显著差异。

Identification of the in vitro HIV-2/SIV RNA dimerization site reveals striking differences with HIV-1.

作者信息

Jossinet F, Lodmell J S, Ehresmann C, Ehresmann B, Marquet R

机构信息

Institut de Biologie Moléculaire et Cellulaire, UPR 9002 du CNRS, 15 rue René Descartes, 67084 Strasbourg, France.

出版信息

J Biol Chem. 2001 Feb 23;276(8):5598-604. doi: 10.1074/jbc.M008642200. Epub 2000 Nov 22.

DOI:10.1074/jbc.M008642200
PMID:11092889
Abstract

Although their genomes cannot be aligned at the nucleotide level, the HIV-1/SIVcpz and the HIV-2/SIVsm viruses are closely related lentiviruses that contain homologous functional and structural RNA elements in their 5'-untranslated regions. In both groups, the domains containing the trans-activating region, the 5'-copy of the polyadenylation signal, and the primer binding site (PBS) are followed by a short stem-loop (SL1) containing a six-nucleotide self-complementary sequence in the loop, flanked by unpaired purines. In HIV-1, SL1 is involved in the dimerization of the viral RNA, in vitro and in vivo. Here, we tested whether SL1 has the same function in HIV-2 and SIVsm RNA. Surprisingly, we found that SL1 is neither required nor involved in the dimerization of HIV-2 and SIV RNA. We identified the NarI sequence located in the PBS as the main site of HIV-2 RNA dimerization. cis and trans complementation of point mutations indicated that this self-complementary sequence forms symmetrical intermolecular interactions in the RNA dimer and suggested that HIV-2 and SIV RNA dimerization proceeds through a kissing loop mechanism, as previously shown for HIV-1. Furthermore, annealing of tRNA(3)(Lys) to the PBS strongly inhibited in vitro RNA dimerization, indicating that, in vivo, the intermolecular interaction involving the NarI sequence must be dissociated to allow annealing of the primer tRNA.

摘要

尽管HIV-1/SIVcpz和HIV-2/SIVsm病毒的基因组在核苷酸水平上无法比对,但它们是密切相关的慢病毒,在其5'-非翻译区含有同源的功能和结构RNA元件。在这两组病毒中,包含反式激活区、多聚腺苷酸化信号的5'-拷贝以及引物结合位点(PBS)的结构域之后是一个短茎环(SL1),其环中含有一个六核苷酸的自我互补序列,两侧为未配对的嘌呤。在HIV-1中,SL1在体外和体内都参与病毒RNA的二聚化。在此,我们测试了SL1在HIV-2和SIVsm RNA中是否具有相同功能。令人惊讶的是,我们发现SL1对于HIV-2和SIV RNA的二聚化既不是必需的,也不参与其中。我们确定位于PBS中的NarI序列是HIV-2 RNA二聚化的主要位点。点突变的顺式和反式互补表明,这个自我互补序列在RNA二聚体中形成对称的分子间相互作用,并提示HIV-2和SIV RNA二聚化通过亲吻环机制进行,正如之前在HIV-1中所显示的那样。此外,tRNA3(Lys)与PBS的退火强烈抑制了体外RNA二聚化,表明在体内,涉及NarI序列的分子间相互作用必须解离,以允许引物tRNA退火。

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