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Functional analysis of the tick-borne encephalitis virus cyclization elements indicates major differences between mosquito-borne and tick-borne flaviviruses

机译:the传脑炎病毒环化成分的功能分析表明蚊传黄病毒和tick传黄病毒之间的主要区别

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摘要

The linear, positive-stranded RNA genome of flaviviruses is thought to adopt a circularized conformation via interactions of short complementary sequence elements located within its terminal regions. This process of RNA cyclization is a crucial precondition for RNA replication. In the case of mosquito-borne flaviviruses, highly conserved cyclization sequences (CS) have been identified, and their functionality has been experimentally confirmed. Here, we provide an experimental identification of CS elements of tick-borne encephalitis virus (TBEV). These elements, termed 5'-CS-A and 3'-CS-A, are conserved among various tick-borne flaviviruses, but they are unrelated to the mosquito-borne CS elements and are located at different genomic positions. The 5'-CS-A element is situated upstream rather than downstream of the AUG start codon and, in contrast to mosquito-borne flaviviruses, it was found that the entire protein C coding region is not essential for TBEV replication. The complementary 3'-CS-A element is located within the bottom stem rather than upstream of the characteristic 3'-terminal stem-loop structure, implying that this part of the proposed structure cannot be formed when the genome is in its circularized conformation. Finally, we demonstrate that the CS-A elements can also mediate their function when the 5'-CS-A element is moved from its natural position to one corresponding to the mosquito-borne CS. The recognition of essential RNA elements and their differences between mosquito-borne and tick-borne flaviviruses has practical implications for the design of replicons in vaccine and vector development. Copyright Π2006, American Society for Microbiology. All Rights Reserved.
机译:黄病毒的线性正链RNA基因组被认为是通过位于其末端区域内的短互补序列元件的相互作用而采用了环化构象。 RNA环化的过程是RNA复制的关键前提。对于蚊媒黄病毒,已鉴定出高度保守的环化序列(CS),并已通过实验证实其功能。在这里,我们提供tick传脑炎病毒(TBEV)的CS元素的实验鉴定。这些被称为5'-CS-A和3'-CS-A的元件在各种壁虱传播的黄病毒中是保守的,但与蚊子传播的CS元件无关,并且位于不同的基因组位置。 5'-CS-A元件位于AUG起始密码子的上游而不是下游,并且与蚊子传播的黄病毒相反,发现整个蛋白C编码区对于TBEV复制不是必需的。互补的3'-CS-A元件位于底部茎中,而不是特征性3'-末端茎-环结构的上游,这意味着当基因组处于其环化构象时,无法形成所提议结构的这一部分。最后,我们证明了当5'-CS-A元素从其自然位置移动到对应于蚊媒CS的一个位置时,CS-A元素也可以介导其功能。蚊子传播的黄病毒和avi传播的黄病毒之间必需的RNA元件及其差异的识别对疫苗和载体开发中复制子的设计具有实际意义。版权所有©2006,美国微生物学会。版权所有。

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