1型牛乳头瘤病毒晚期特异性核苷酸3605的3'剪接位点的利用受一种新型外显子双组分调节因子调控,而非受内含子富含嘌呤元件的调控。
Utilization of the bovine papillomavirus type 1 late-stage-specific nucleotide 3605 3' splice site is modulated by a novel exonic bipartite regulator but not by an intronic purine-rich element.
作者信息
Zheng Z M, Reid E S, Baker C C
机构信息
Basic Research Laboratory, Division of Basic Sciences, National Cancer Institute, National Institutes of Health, Bethesda, Maryland 20892, USA.
出版信息
J Virol. 2000 Nov;74(22):10612-22. doi: 10.1128/jvi.74.22.10612-10622.2000.
Bovine papillomavirus type 1 (BPV-1) late gene expression is regulated at both transcriptional and posttranscriptional levels. Maturation of the capsid protein (L1) pre-mRNA requires a switch in 3' splice site utilization. This switch involves activation of the nucleotide (nt) 3605 3' splice site, which is utilized only in fully differentiated keratinocytes during late stages of the virus life cycle. Our previous studies of the mechanisms that regulate BPV-1 alternative splicing identified three cis-acting elements between these two splice sites. Two purine-rich exonic splicing enhancers, SE1 and SE2, are essential for preferential utilization of the nt 3225 3' splice site at early stages of the virus life cycle. Another cis-acting element, exonic splicing suppressor 1 (ESS1), represses use of the nt 3225 3' splice site. In the present study, we investigated the late-stage-specific nt 3605 3' splice site and showed that it has suboptimal features characterized by a nonconsensus branch point sequence and a weak polypyrimidine track with interspersed purines. In vitro and in vivo experiments showed that utilization of the nt 3605 3' splice site was not affected by SE2, which is intronically located with respect to the nt 3605 3' splice site. The intronic location and sequence composition of SE2 are similar to those of the adenovirus IIIa repressor element, which has been shown to inhibit use of a downstream 3' splice site. Further studies demonstrated that the nt 3605 3' splice site is controlled by a novel exonic bipartite element consisting of an AC-rich exonic splicing enhancer (SE4) and an exonic splicing suppressor (ESS2) with a UGGU motif. Functionally, this newly identified bipartite element resembles the bipartite element composed of SE1 and ESS1. SE4 also functions on a heterologous 3' splice site. In contrast, ESS2 functions as an exonic splicing suppressor only in a 3'-splice-site-specific and enhancer-specific manner. Our data indicate that BPV-1 splicing regulation is very complex and is likely to be controlled by multiple splicing factors during keratinocyte differentiation.
牛乳头瘤病毒1型(BPV-1)晚期基因表达在转录和转录后水平均受到调控。衣壳蛋白(L1)前体mRNA的成熟需要3'剪接位点利用的转换。这种转换涉及核苷酸(nt)3605 3'剪接位点的激活,该位点仅在病毒生命周期后期的完全分化角质形成细胞中被利用。我们之前对调控BPV-1可变剪接机制的研究确定了这两个剪接位点之间的三个顺式作用元件。两个富含嘌呤的外显子剪接增强子SE1和SE2,对于病毒生命周期早期nt 3225 3'剪接位点的优先利用至关重要。另一个顺式作用元件,外显子剪接抑制因子1(ESS1),抑制nt 3225 3'剪接位点的使用。在本研究中,我们研究了晚期特异性的nt 3605 3'剪接位点,发现它具有次优特征,其特点是分支点序列不一致且多嘧啶序列较弱,中间穿插着嘌呤。体外和体内实验表明,nt 3605 3'剪接位点的利用不受SE2的影响,SE2相对于nt 3605 3'剪接位点位于内含子中。SE2的内含子位置和序列组成与腺病毒IIIa抑制元件相似,后者已被证明可抑制下游3'剪接位点的使用。进一步研究表明,nt 3605 3'剪接位点受一个新的外显子二分元件控制,该元件由富含AC的外显子剪接增强子(SE4)和具有UGGU基序的外显子剪接抑制因子(ESS2)组成。在功能上,这个新鉴定的二分元件类似于由SE1和ESS1组成的二分元件。SE4也作用于异源3'剪接位点。相反,ESS2仅以3'剪接位点特异性和增强子特异性方式作为外显子剪接抑制因子发挥作用。我们的数据表明,BPV-1剪接调控非常复杂,可能在角质形成细胞分化过程中受多种剪接因子控制。
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