人类免疫缺陷病毒1型(HIV-1)tat外显子2内的剪接调控元件是M组HIV-1毒株的特征,但不是O组HIV-1毒株的特征。
Splicing regulatory elements within tat exon 2 of human immunodeficiency virus type 1 (HIV-1) are characteristic of group M but not group O HIV-1 strains.
作者信息
Bilodeau P S, Domsic J K, Stoltzfus C M
机构信息
Department of Microbiology, Program in Molecular Biology, University of Iowa, Iowa City, Iowa 52242, USA.
出版信息
J Virol. 1999 Dec;73(12):9764-72. doi: 10.1128/JVI.73.12.9764-9772.1999.
In the NL4-3 strain of human immunodeficiency virus type 1 (HIV-1), regulatory elements responsible for the relative efficiencies of alternative splicing at the tat, rev, and the env/nef 3' splice sites (A3 through A5) are contained within the region of tat exon 2 and its flanking sequences. Two elements affecting splicing of tat, rev, and env/nef mRNAs have been localized to this region. First, an exon splicing silencer (ESS2) in NL4-3, located approximately 70 nucleotides downstream from the 3' splice site used to generate tat mRNA, acts specifically to inhibit splicing at this splice site. Second, the A4b 3' splice site, which is the most downstream of the three rev 3' splice sites, also serves as an element inhibiting splicing at the env/nef 3' splice site A5. These elements are conserved in some but not all HIV-1 strains, and the effects of these sequence changes on splicing have been investigated in cell transfection and in vitro splicing assays. SF2, another clade B virus and member of the major (group M) viruses, has several sequence changes within ESS2 and uses a different rev 3' splice site. However, splicing is inhibited by the two elements similarly to NL4-3. As with the NL4-3 strain, the SF2 A4b AG dinucleotide overlaps an A5 branchpoint, and thus the inhibitory effect may result from competition of the same site for two different splicing factors. The sequence changes in ANT70C, a member of the highly divergent outlier (group O) viruses, are more extensive, and ESS2 activity in tat exon 2 is not present. Group O viruses also lack the rev 3' splice site A4b, which is conserved in all group M viruses. Mutagenesis of the most downstream rev 3' splice site of ANT70C does not increase splicing at A5, and all of the branchpoints are upstream of the two rev 3' splice sites. Thus, splicing regulatory elements in tat exon 2 which are characteristic of most group M HIV-1 strains are not present in group O HIV-1 strains.
在1型人类免疫缺陷病毒(HIV-1)的NL4-3毒株中,负责tat、rev以及env/nef 3'剪接位点(A3至A5)可变剪接相对效率的调控元件包含在tat外显子2区域及其侧翼序列内。已将影响tat、rev和env/nef mRNA剪接的两个元件定位到该区域。首先,NL4-3中的一个外显子剪接沉默子(ESS2),位于用于产生tat mRNA的3'剪接位点下游约70个核苷酸处,特异性地抑制该剪接位点的剪接。其次,A4b 3'剪接位点是rev的三个3'剪接位点中最下游的一个,它也作为一个抑制env/nef 3'剪接位点A5剪接的元件。这些元件在一些但并非所有HIV-1毒株中保守,并且已在细胞转染和体外剪接试验中研究了这些序列变化对剪接的影响。SF2是另一种B亚型病毒且是主要(M组)病毒的成员,在ESS2内有几个序列变化,并使用不同的rev 3'剪接位点。然而,这两个元件对剪接的抑制作用与NL4-3相似。与NL4-3毒株一样,SF2的A4b AG二核苷酸与A5分支点重叠,因此抑制作用可能是由于同一位点竞争两种不同的剪接因子所致。高度分化的异常病毒(O组)成员ANT70C中的序列变化更为广泛,tat外显子2中不存在ESS2活性。O组病毒也缺乏在所有M组病毒中保守的rev 3'剪接位点A4b。对ANT70C最下游的rev 3'剪接位点进行诱变不会增加A5处的剪接,并且所有分支点都在两个rev 3'剪接位点的上游。因此,大多数M组HIV-1毒株特有的tat外显子2中的剪接调控元件在O组HIV-1毒株中不存在。
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