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The first pre-rRNA-processing event occurs in a large complex: analysis by gel retardation, sedimentation, and UV cross-linking.

机译:第一个rRNA预处理过程发生在一个大型复合物中:通过凝胶阻滞,沉降和UV交联进行分析。

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摘要

The first processing event that mouse pre-rRNA undergoes occurs within the external transcribed spacer and is efficiently reproduced in vitro. Analysis with nondenaturing polyacrylamide gels revealed the formation of heparin-resistant complexes of retarded electrophoretic mobility on the substrate rRNA. The specificity of these complexes was demonstrated by their elimination due to competition with processing-competent, but not with processing-incompetent, rRNAs. Furthermore, complex formation, like the processing cleavage, required only 28 nucleotides of rRNA sequence adjacent to the processing site but was stimulated by additional downstream conserved sequences. These processing complexes formed in a time-dependent manner, and once assembled, they were stable to challenge by competitor rRNA and remained on the processed rRNA. Their sedimentation coefficient was approximately 20S. UV cross-linking studies with 4-thiouridine-substituted rRNA have identified six polypeptides, 52 to 250 kilodaltons, that are specifically bound to the rRNA processing substrate.
机译:小鼠pre-rRNA经历的第一个加工事件发生在外部转录的间隔区中,并在体外有效繁殖。用非变性聚丙烯酰胺凝胶进行的分析显示,底物rRNA上肝素抗性复合物的电泳迁移率降低。这些复合物的特异性通过与加工能力而非竞争能力的rRNA竞争而被消除而得以证明。此外,复杂的形成,如加工切割,仅需要28个核苷酸的rRNA序列与加工位点相邻,但会受到其他下游保守序列的刺激。这些加工复合物以时间依赖性的方式形成,并且一旦组装,它们就稳定地被竞争者rRNA挑战,并保留在加工的rRNA上。它们的沉降系数约为20S。用4-硫尿苷取代的rRNA进行的UV交联研究已鉴定出52至250公里道尔顿的六种多肽,它们特异性结合到rRNA加工底物上。

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