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In Vivo Packaging of Brome Mosaic Virus RNA3 but Not RNAs 1 and 2 Is Dependent on a cis-Acting 3′ tRNA-Like Structure

机译:凤梨花叶病毒RNA3的体内包装而不是RNA 1和2取决于顺式作用的3tRNA样结构。

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摘要

The four encapsidated RNAs of brome mosaic virus (BMV; B1, B2, B3, and B4) contain a highly conserved 3′ 200-nucleotide (nt) region encompassing the tRNA-like structure (TLS) which is required for packaging in vitro (Y. G. Choi, T. W. Dreher, and A. L. N. Rao, Proc. Natl. Acad. Sci. USA 99:655-660, 2002). To validate these observations in vivo, we performed packaging assays using Agrobacterium-mediated transient expression of RNAs and coat protein (CP) (P. Annamalai and A. L. N. Rao, Virology 338:96-111, 2005). Coexpression of TLS-less constructs of B1 or B2 or B3 and CP mRNAs in Nicotiana benthamiana leaves resulted in packaging of TLS-less B1 and B2 but not B3, suggesting that packaging of B3 requires the TLS in cis. This conjecture was confirmed by the efficient packaging of a B3 chimera in which the viral TLS was replaced with a cellular tRNATyr. When N. benthamiana leaves were infiltrated with a mixture of transformants containing wild-type B1 (wtB1) plus wtB2 plus a TLS-less B3 (wtB1+wtB2+TLS-lessB3), the 3′ end of progeny B3 was restored by heterologous recombination with that of either B1 or B2. This intrinsic cis-requirement of TLS in promoting B3 packaging was further confirmed when a mixture containing agrotransformants of TLS-less B1+B2+B3 was supplemented with either wtB4 or a 3′ 200-nt or 3′ 336-nt untranslated region (UTR) of B3. Northern blot analysis followed by sequencing of B3 progeny revealed that replication of TLS-less B3, but not TLS-less B1 or B2, was fully restored due to recombination with TLS from transiently expressed wtB4 or the B3 3′ UTR. Collectively, these observations suggested that the requirement of a cis-acting TLS is distinct for B3 compared with B1 or B2.
机译:溴化花叶病毒(BMV; B1,B2,B3和B4)的四个衣壳化RNA包含高度保守的3'200核苷酸(nt)区,其中包含tRNA样结构(TLS),这是体外包装所需的(TLS) YG Choi,TW Dreher,和ALN Rao,Proc.Natl.Acad.Sci.USA 99:655-660,2002)。为了在体内验证这些观察结果,我们使用农杆菌介导的RNA和外壳蛋白(CP)瞬时表达进行包装测定(P. Annamalai和A. L. N. Rao,病毒学338:96-111,2005)。 B1或B2或B3的无TLS少的构建体与CP mRNA在烟草中的共表达会导致无TLS的B1和B2而不是B3的包装,这表明B3的包装需要TLS顺式。 B3嵌合体的有效包装证实了这一推测,其中病毒TLS被细胞tRNA Tyr 代替。当本塞姆氏烟草叶片被含有野生型B1(wtB1)+ wtB2加上无TLS的B3(wtB1 + wtB2 + TLS-lessB3)的转化体混合物浸润后,子代B3的3'端通过异源重组而恢复与B1或B2相同。当向含有无TLS的B1 + B2 + B3的农业转化子的混合物中添加wtB4或3'200-nt或3'336-nt非翻译区(UTR)时,进一步证实了TLS在促进B3包装方面的内在顺式要求。 )。 Northern印迹分析,然后对B3后代进行测序,结果表明,由于与TLS重组,瞬时表达的wtB4或B3 3'UTR与TLS重组,使无TLS的B3而不是无TLS的B1或B2的复制得以完全恢复。总体而言,这些观察结果表明,与B1或B2相比,B3对顺式作用TLS的要求不同。

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