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Multiple Cis-acting elements modulate programmed-1 ribosomal frameshifting in Pea enation mosaic virus

机译:豌豆花叶病毒中多个顺式作用元件调节程序化1核糖体移码

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Programmed -1 ribosomal frameshifting (-1 PRF) is used by many positive-strand RNA viruses for translation of required products. Despite extensive studies, it remains unresolved how cis-elements just downstream of the recoding site promote a precise level of frameshifting. The Umbravirus Pea enation mosaic virus RNA2 expresses its RNA polymerase by -1 PRF of the 5'-proximal ORF (p33). Three hairpins located in the vicinity of the recoding site are phylogenetically conserved among Umbraviruses. The central Recoding Stimulatory Element (RSE), located downstream of the p33 termination codon, is a large hairpin with two asymmetric internal loops. Mutational analyses revealed that sequences throughout the RSE and the RSE lower stem (LS) structure are important for frameshifting. SHAPE probing of mutants indicated the presence of higher order structure, and sequences in the LS may also adapt an alternative conformation. Long-distance pairing between the RSE and a 3' terminal hairpin was less critical when the LS structure was stabilized. A basal level of frameshifting occurring in the absence of the RSE increases to 72% of wild-type when a hairpin upstream of the slippery site is also deleted. These results suggest that suppression of frameshifting may be needed in the absence of an active RSE conformation.
机译:许多正链RNA病毒都使用程序-1核糖体移码(-1 PRF)来翻译所需的产物。尽管进行了广泛的研究,但仍未解决正好位于记录位点下游的顺式元件如何促进精确水平的移码。伞病毒豌豆花叶病毒RNA2通过5'-近端ORF的-1 PRF(p33)表达其RNA聚合酶。在编码病毒中,位于记录位点附近的三个发夹在系统发育上是保守的。中央编码刺激元件(RSE)位于p33终止密码子的下游,是一个带有两个不对称内部环的大发夹。突变分析显示,整个RSE和RSE下茎(LS)结构中的序列对于移码都很重要。突变体的SHAPE探测表明存在更高阶的结构,并且LS中的序列也可能适应其他构象。当LS结构稳定时,RSE和3'末端发夹之间的长距离配对不太重要。当滑点上游的发夹也被删除时,在不存在RSE的情况下发生的基本移码水平增加到野生型的72%。这些结果表明,在没有有效的RSE构象的情况下,可能需要抑制移码。

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