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莫洛尼鼠白血病病毒基因组RNA中RNA-RNA连接的初步物理图谱分析。

Preliminary physical mapping of RNA-RNA linkages in the genomic RNA of Moloney murine leukemia virus.

作者信息

Hibbert Catherine S, Rein Alan

机构信息

HIV Drug Resistance Program, National Cancer Institute--Frederick, P.O. Box B, Frederick, Maryland 21702-1201, USA.

出版信息

J Virol. 2005 Jul;79(13):8142-8. doi: 10.1128/JVI.79.13.8142-8148.2005.

Abstract

Retrovirus particles contain two copies of their genomic RNA, held together in a dimer by linkages which presumably consist of a limited number of base pairs. In an effort to localize these linkages, we digested deproteinized RNA from Moloney murine leukemia virus (MLV) particles with RNase H in the presence of oligodeoxynucleotides complementary to specific sites in viral RNA. The cleaved RNAs were then characterized by nondenaturing gel electrophoresis. We found that fragments composed of nucleotides 1 to 754 were dimeric, with a linkage as thermostable as that between dimers of intact genomic RNA. In contrast, there was no stable linkage between fragments consisting of nucleotides 755 to 8332. Thus, the most stable linkage between monomers is on the 5' side of nucleotide 754. This conclusion is in agreement with earlier electron microscopic analyses of partially denatured viral RNAs and with our study (C. S. Hibbert, J. Mirro, and A. Rein, J. Virol. 78:10927-10938, 2004) of encapsidated nonviral mRNAs containing inserts of viral sequence. We obtained similar results with RNAs from immature MLV particles, in which the dimeric linkage is different from that in mature particles and has not previously been localized. The 5' and 3' fragments of cleaved RNA are all held together by thermolabile linkages, indicating the presence of tethering interactions between bases 5' and bases 3' of the cleavage site. When RNAs from mature particles were cleaved at nucleotide 1201, we detected tethering interactions spanning the cleavage site which are intramonomeric and are as strong as the most stable linkage between the monomers.

摘要

逆转录病毒颗粒含有两份基因组RNA,它们通过可能由有限数量碱基对组成的连接形成二聚体。为了确定这些连接的位置,我们在与病毒RNA中特定位点互补的寡聚脱氧核苷酸存在下,用RNase H消化莫洛尼鼠白血病病毒(MLV)颗粒中的脱蛋白RNA。然后通过非变性凝胶电泳对切割后的RNA进行表征。我们发现,由核苷酸1至754组成的片段是二聚体,其连接的热稳定性与完整基因组RNA二聚体之间的连接相同。相比之下,由核苷酸755至8332组成的片段之间没有稳定的连接。因此,单体之间最稳定的连接位于核苷酸754的5'侧。这一结论与早期对部分变性病毒RNA的电子显微镜分析以及我们对含有病毒序列插入片段的衣壳化非病毒mRNA的研究(C.S.希伯特、J.米罗和A.莱茵,《病毒学杂志》78:10927 - 10938,2004年)一致。我们从未成熟MLV颗粒的RNA中获得了类似的结果,其中二聚体连接与成熟颗粒中的不同,且此前尚未定位。切割后RNA的5'和3'片段均通过热不稳定连接结合在一起,表明切割位点的5'碱基和3'碱基之间存在系留相互作用。当成熟颗粒的RNA在核苷酸1201处切割时,我们检测到跨越切割位点的系留相互作用,这些相互作用是单体内部的,并且与单体之间最稳定的连接一样强。

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