Skulachev M V, Ivanov P A, Karpova O V, Korpela T, Rodionova N P, Dorokhov Y L, Atabekov J G
Department of Virology, Moscow State University, Moscow, 119899, Russia.
Virology. 1999 Oct 10;263(1):139-54. doi: 10.1006/viro.1999.9928.
Previously we reported that, unlike RNA of typical tobamoviruses, the translation of the coat protein (CP) gene of a crucifer-infecting tobamovirus (crTMV) in vitro occurred by an internal ribosome entry mechanism mediated by the 148-nt region that contained an internal ribosome entry site (IRES(CP,148)(CR)). The equivalent 148-nt sequence from TMV U1 RNA (U1(CP,148)(SP)) was incapable of promoting internal initiation. In the present work, we have found that the 228-nt region upstream of the movement protein (MP) gene of crTMV RNA (IRES(MP,228)(CR)) contained an IRES element that directed in vitro translation of the 3'-proximal reporter genes from chimeric dicistronic transcripts. Surprisingly, the equivalent 228-nt sequence upstream from the MP gene of TMV U1 directed translation of the downstream gene of a dicistronic transcripts as well. Consequently this sequence was termed IRES(MP,228)(U1). It was shown that IRES(MP,228)(CR), IRES(MP,228)(U1), and IRES(CP,148)(CR) could mediate expression of the 3'-proximal GUS gene from dicistronic 35S promoter-based constructs in vivo in experiments on transfection of tobacco protoplasts and particle bombardment of Nicotiana benthamiana leaves. The results indicated that an IRES element was located within the 75-nt region upstream of MP gene (IRES(MP,75)), which corresponded closely to the length of the 5'UTR of TMV subgenomic RNA (sgRNA) I(2). The RNA transcripts structurally equivalent to I(2) sgRNAs of TMV U1 and crTMV, but containing a hairpin structure (H) immediately upstream of IRES(MP,75) (HIRES(MP), (75)(CR)-MP-CP-3'UTR; HIRES(MP,75)(U1)-MP-CP-3'UTR), were able to express the MP gene in vitro. The capacity of HIRES(MP,75)(CR) sequence for mediating internal translation of the 3'-proximal GUS gene in vivo, in tobacco protoplasts, was demonstrated. We suggested that expression of the MP gene from I(2) sgRNAs might proceed via internal ribosome entry pathway mediated by IRES(MP) element contained in the 75-nt 5'UTR. Our results admit that a ribosome scanning mechanism of the MP gene expression from I(2) sgRNA operates concurrently.
先前我们报道,与典型烟草花叶病毒的RNA不同,一种十字花科感染烟草花叶病毒(crTMV)的外壳蛋白(CP)基因在体外的翻译是通过由148个核苷酸区域介导的内部核糖体进入机制进行的,该区域包含一个内部核糖体进入位点(IRES(CP,148)(CR))。来自烟草花叶病毒U1 RNA的等效148个核苷酸序列(U1(CP,148)(SP))无法促进内部起始。在本研究中,我们发现crTMV RNA运动蛋白(MP)基因上游的228个核苷酸区域(IRES(MP,228)(CR))包含一个IRES元件,该元件指导嵌合双顺反子转录本中3'-近端报告基因的体外翻译。令人惊讶的是,烟草花叶病毒U1的MP基因上游的等效228个核苷酸序列也指导双顺反子转录本下游基因的翻译。因此,该序列被称为IRES(MP,228)(U1)。结果表明,IRES(MP,228)(CR)、IRES(MP,228)(U)和IRES(CP,148)(CR)在烟草原生质体转染和本氏烟草叶片粒子轰击实验中,能够在体内介导基于双顺反子35S启动子构建体中3'-近端GUS基因的表达。结果表明,一个IRES元件位于MP基因上游的75个核苷酸区域内(IRES(MP,75)),这与烟草花叶病毒亚基因组RNA(sgRNA)I(2)的5'UTR长度密切对应。与烟草花叶病毒U1和crTMV的I(2) sgRNAs结构等效,但在IRES(MP,75)上游紧邻一个发夹结构(H)的RNA转录本(HIRES(MP),(75)(CR)-MP-CP-3'UTR;HIRES(MP,75)(U1)-MP-CP-3'UTR)能够在体外表达MP基因。证明了HIRES(MP,75)(CR)序列在烟草原生质体中体内介导3'-近端GUS基因内部翻译的能力。我们认为,I(2) sgRNAs中MP基因的表达可能通过由75个核苷酸5'UTR中包含的IRES(MP)元件介导的内部核糖体进入途径进行。我们的结果承认,I(2) sgRNA中MP基因表达的核糖体扫描机制同时起作用。
Zotero 插件