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Messenger RNA processing and nuclear structure: isolation of nuclear ribonucleoprotein particles containing beta-globin messenger RNA precursors

机译:Messenger RNA加工和核结构:分离含有β-珠蛋白信使RNA前体的核糖核蛋白颗粒

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摘要

To explore the relationships between transcription, messenger RNA (mRNA) processing, and nuclear structure, ribonucleoprotein particles containing heterogeneous nuclear RNA (hnRNP) have been purified from globin-producing mouse Friend erythroleukemia cells. These nuclear hnRNP particles sediment at 50S-200S and contain, in addition to high molecular weight hnRNA, a specific set of nuclear proteins predominated by a major component of approximately 38,000 mol wt. The hnRNP particles are free of histones and ribosomal structural proteins, indicating their purification from the two other major nucleoprotein components of the nucleus: chromatin and nucleolar ribosomal precursor RNP particles. Th authenticity of the Friend cell hnRNP particles is demonstrated by the results of reconstruction experiments with deproteinized hnRNA, and by the resistance of the articles to dissociation during isopycnic banding in Cs2SO4 gradients without prior aldehyde fixation. Hybridization analysis with cloned mouse beta-globin DNA demonstrates that hnRNP particles from induced Friend cells contain newly synthesized transcripts of the beta-globin gene. Agarose gel electrophoresis of hnRNP particle-derived RNA denatured in glyoxal followed by "Northern" transfer to diazobenzyloxymethyl paper and hybridization with 32P-labeled cloned mouse beta-globin DNA reveals the presence in hnRNP of two size classes of beta-globin gene transcripts, the larger of which corresponds to the pre-spliced 15S beta-globin mRNA precursor previously identified in whole nuclear RNA, and the smaller of which corresponds to completely processed 9S beta-globin mRNA. These results establish, for the first time, that the nuclear transcripts of a specific, well-defined eukaryotic structural gene can be isolated in an RNP particle form, and that their RNP structure persists throughout mRNA splicing.
机译:为了探索转录,信使RNA(mRNA)加工与核结构之间的关系,已从产生球蛋白的小鼠Friend erythreu白血病血细胞中纯化了含有异质核RNA(hnRNP)的核糖核蛋白颗粒。这些核hnRNP颗粒在50S-200S处沉淀,除了高分子量hnRNA外,还含有一组特定的核蛋白,主要成分约为38,000 mol wt。 hnRNP颗粒不含组蛋白和核糖体结构蛋白,表明它们已从细胞核的两个其他主要核蛋白成分中纯化:染色质和核仁核糖体前体RNP颗粒。 Friend细胞hnRNP颗粒的真实性通过脱蛋白hnRNA的重建实验结果证明,并且在不进行醛固定的情况下,通过在Cs2SO4梯度的等密度带中制品对解离的抵抗力得到了证明。用克隆的小鼠β-珠蛋白DNA进行的杂交分析表明,来自诱导的Friend细胞的hnRNP颗粒含有新合成的β-珠蛋白基因的转录本。乙二醛中变性的hnRNP颗粒来源的RNA的琼脂糖凝胶电泳,然后“北方”转移至重氮苄氧基甲基纸,并与32P标记的克隆的小鼠β-珠蛋白DNA杂交,揭示了hnRNP中存在两种大小的β-珠蛋白基因转录本,其中较大的对应于先前在全核RNA中鉴定的预剪接的15Sβ-珠蛋白mRNA前体,较小的对应于完全加工的9Sβ-珠蛋白mRNA。这些结果首次确定了可以RNP颗粒形式分离出一个特定的,定义明确的真核结构基因的核转录本,并且它们的RNP结构在整个mRNA剪接过程中仍然存在。

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