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Subnuclear localization and dynamics of the pre-mRNA 3 ' end processing factor mammalian cleavage factor I 68-kDa subunit

机译:前mRNA 3'末端加工因子哺乳动物卵裂因子I 68-kDa亚基的亚核定位和动力学

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摘要

Mammalian cleavage factor I (CF I-m) is an essential factor that is required for the first step in pre-mRNA 3' end processing. Here, we characterize CF I(m)68 subnuclear distribution and mobility. Fluorescence microscopy reveals that in addition to paraspeckles CF Im68 accumulates in structures that partially overlap with nuclear speckles. Analysis of synchronized cells shows that CF I(m)68 distribution in speckles and paraspeckles varies during the cell cycle. At an ultrastructural level, CF Im68 is associated with perichromatin fibrils, the sites of active transcription, and concentrates in interchromatin granules-associated zones. We show that CF I(m)68 colocalizes with bromouridine, RNA polymerase II, and the splicing factor SC35. On inhibition of transcription, endogenous CF I(m)68 no longer associates with perichromatin fibrils, but it can still be detected in interchromatin granules-associated zones. These observations support the idea that not only splicing but also 3' end processing occurs cotranscriptionally. Finally, fluorescence recovery after photobleaching analysis reveals that the CF Im68 fraction associated with paraspeckles moves at a rate similar to the more dispersed molecules in the nucleoplasm, demonstrating the dynamic nature of this compartment. These findings suggest that paraspeckles are a functional compartment involved in RNA metabolism in the cell nucleus.
机译:哺乳动物卵裂因子I(CF I-m)是mRNA前3'末端加工第一步所需的重要因子。在这里,我们表征CF I(m)68亚核的分布和迁移率。荧光显微镜显示,除了斑点外,CF Im68还在与核斑点部分重叠的结构中积累。对同步化细胞的分析表明,散斑和副散斑中的CF I(m)68分布在细胞周期中发生变化。在超微结构水平上,CF Im68与染色质周染色质原纤维,活跃的转录位点相关,并集中在染色质间颗粒相关区域。我们显示CF I(m)68与溴尿苷,RNA聚合酶II和剪接因子SC35共定位。抑制转录后,内源性CF I(m)68不再与染色质原纤维结合,但仍可以在染色质间颗粒相关区域中检测到。这些观察结果支持这样的想法,即不仅剪接而且3'末端加工也共转录发生。最后,光漂白分析后的荧光恢复表明,与副斑点相关的CF Im68组分以类似于核质中更分散的分子的速率移动,证明了该区室的动态性质。这些发现表明,散斑是参与细胞核中RNA代谢的功能区室。

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