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The packaging signal of influenza viral RNA molecules.

机译:流感病毒RNA分子的包装信号。

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The packaging signal present in influenza viral RNA molecules is shown not to constitute a separate structural element, but to reside within the 5'-bulged promoter structure, as caused by the central unpaired residue A10 in its 5' branch. Upon insertion of two uridine residues in the 3' branch opposite A10, the minus-strand viral RNA (vRNA) promoter is converted into a 3'-bulged structure, whereas the plus-strand cRNA promoter instead adopts the 5'-bulged conformation. In this promoter variant it is exclusively the cRNA that is found packaged in the progeny virions. Upon insertion of only a single uridine nucleotide opposite 5'A10, the two debulged structures of the vRNA and cRNA promoters are rendered identical, and both vRNA and cRNA molecules are packaged indiscriminately, in a 1:1 ratio, but at lower rates. We propose that the binding interactions of viral polymerase with either of the two differently bulged vRNA and cRNA promoter structures result in two different conformations of the enzyme protein. Only the 5' bulged RNA-associated polymerase conformation appears to be recognized for nuclear export, which depends on nuclear matrix protein M1 and nonstructural protein NS2. And the respective wild-type vRNP- or insertion mutant cRNP complex is observed to enter the cytoplasm and hence is included in the viral encapsidation process, which takes place at the plasma membrane.
机译:流感病毒RNA分子中存在的包装信号显示不构成单独的结构元件,而是驻留在5'突出的启动子结构中,这是由其5'分支中未配对的中央残基A10引起的。在A10对面的3'分支中插入两个尿苷残基后,负链病毒RNA(vRNA)启动子转换为3'凸起结构,而正链cRNA启动子则采用5'凸起构象。在该启动子变体中,仅cRNA被包装在子代病毒体中。当仅插入一个与5'A10相反的尿苷核苷酸时,vRNA和cRNA启动子的两个残基结构相同,vRNA和cRNA分子均以1:1的比例随意包装,但比率较低。我们建议病毒聚合酶与两个不同鼓胀的vRNA和cRNA启动子结构中的一个的结合相互作用导致酶蛋白的两个不同构象。似乎只有5'凸起的与RNA相关的聚合酶构象可用于核输出,这取决于核基质蛋白M1和非结构蛋白NS2。并且观察到相应的野生型vRNP-或插入突变体cRNP复合物进入细胞质,因此被包括在质膜中发生的病毒衣壳化过程中。

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