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3' processing of pre-mRNA plays a major role in proliferation-dependent regulation of histone gene expression

机译:前mRNA的3'加工在依赖增殖的组蛋白基因表达调控中起主要作用

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SUMMARY A short histone-like fusion RNA, generated when the RNA 3' processing signal from a mouse histone H4 gene is inserted into a heterologous transcription unit, becomes correctly down-regulated in G1-arrested cells of a temperature-sensitive mouse mastocytoma cell cycle mutant (21-Tb; Stauber et al., EMBO J. 5, 3297–3303 [1986]), due to a specific deficiency in histone RNA processing (Lüscher and Schümperli, EMBO J. 6, 1721–1726 [1987]). In contrast, inhibitors of DNA synthesis, known to stimulate histone mRNA degradation, have little or no effect on the fusion RNA. This RNA can therefore be used to discriminate between regulation by RNA 3' processing and RNA stability, respectively. The fusion RNA is also faithfully regulated in 21-Tb cells arrested in G1 phase by the drug indomethacin or in C127 mouse fibroblasts during a serum starvation experiment. Moreover, nuclear extracts from serum-starved C127 cells show a specific deficiency in a heat-labile component of the histone RNA processing apparatus, similar to that previously observed for temperature-arrested 21-Tb cells. These results suggest that RNA 3' processing is a major determinant for the response of histone mRNA levels to changes in cell proliferation.
机译:概述当将来自小鼠组蛋白H4基因的RNA 3'处理信号插入异源转录单元时,会生成一个短的组蛋白样融合RNA,在温度敏感的小鼠肥大细胞瘤细胞周期的G1阻滞细胞中被正确下调。突变体(21-Tb; Stauber等人,EMBO J. 5,3297–3303 [1986]),由于组蛋白RNA加工中的特定缺陷(Lüscher和Schümperli,EMBO J. 6,1721–1726 [1987])。 。相反,已知刺激组蛋白mRNA降解的DNA合成抑制剂对融合RNA几乎没有影响。因此,该RNA可分别用于区分RNA 3'加工的调控和RNA稳定性。在血清饥饿实验期间,药物吲哚美辛或C127小鼠成纤维细胞在G1期阻滞的21-Tb细胞中也忠实地调节了融合RNA。此外,血清饥饿的C127细胞的核提取物在组蛋白RNA处理设备的热不稳定成分中表现出特定缺陷,类似于先前对温度停滞的21-Tb细胞观察到的缺陷。这些结果表明,RNA 3'加工是组蛋白mRNA水平对细胞增殖变化的响应的主要决定因素。

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