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流感病毒感染细胞中多核糖体相关RNA的表征

Characterization of polysome-associated RNA from influenza virus-infected cells.

作者信息

Nayak D P, D'Andrea E, Wettstein F O

出版信息

J Virol. 1976 Oct;20(1):107-16. doi: 10.1128/JVI.20.1.107-116.1976.

DOI:10.1128/JVI.20.1.107-116.1976
PMID:988191
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC354971/
Abstract

Virus-specific polysome-associated RNA (psRNA) and RNA after dissociation of polysomes were analyzed by direct hybridization with unlabeled viral RNA (vRNA) and complementary RNA (cRNA). psRNA after a 30-min pulse with [3H]uridine contained 28% labeled cRNA, 70% host RNA, and no vRNA. After dissociation, psRNA sedimented heterogeneously. Heavy RNA (greater than 60S), ribosomal subunit RNA (rsuRNA, 30-60S), free mRNA (fmRNA, 10-30S), and light RNA (less than 10S) contained 16%, 54%, 70% and 28% cRNA, respectively, but no vRNA. When actinomycin D (AcD) was added at 2 h postinfection, the nature of the psRNA depended on the concentration of AcD and the condition of the labeling. At AcD concentrations of 1 mug or more per ml, no detectable vRNA or cRNA was associated with polysomes. At 0.2 mug of AcD per ml (a concentration that partially inhibited cRNA synthesis) and 2 h of labeling at 2.5 h postinfection, psRNA contained 40% viral-specific RNA, which included both vRNA and cRNA in almost equal amounts. When polysomes were dissociated, however, viral-specific fm RNA from AcD-treated cells contained exclusively cRNA and no detectable vRNA. Increasing amounts of labeled vRNA were present in the heavy region of the gradient (and in the pellet), which also contained varying amounts of cRNA. The labeled vRNA appears to be associated with polysomes in a cesium chloride density gradient (rho = 1.525 g/ml). Although we have ruled out the trivial explanation of viral ribonucleoprotein contamination,the nature of the complex containing both polysomes and vRNA is unknown.

摘要

通过与未标记的病毒RNA(vRNA)和互补RNA(cRNA)直接杂交,分析了病毒特异性多聚核糖体相关RNA(psRNA)和多聚核糖体解离后的RNA。用[3H]尿苷脉冲标记30分钟后的psRNA含有28%的标记cRNA、70%的宿主RNA,且不含vRNA。解离后,psRNA沉降不均一。重RNA(大于60S)、核糖体亚基RNA(rsuRNA,30 - 60S)、游离mRNA(fmRNA,10 - 30S)和轻RNA(小于10S)分别含有16%、54%、70%和28%的cRNA,但不含vRNA。感染后2小时添加放线菌素D(AcD)时,psRNA的性质取决于AcD的浓度和标记条件。当AcD浓度为每毫升1微克或更高时,多聚核糖体未检测到vRNA或cRNA与之相关。在每毫升0.2微克AcD(该浓度部分抑制cRNA合成)且在感染后2.5小时标记2小时的情况下,psRNA含有40%的病毒特异性RNA,其中vRNA和cRNA几乎等量。然而,当多聚核糖体解离时,来自AcD处理细胞的病毒特异性fm RNA仅含有cRNA,未检测到vRNA。梯度的重区(以及沉淀中)存在越来越多的标记vRNA,其中也含有不同量的cRNA。标记的vRNA似乎以氯化铯密度梯度(ρ = 1.525 g/ml)与多聚核糖体相关。尽管我们排除了病毒核糖核蛋白污染这种简单解释,但包含多聚核糖体和vRNA的复合物的性质尚不清楚。

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本文引用的文献

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