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核仁内核糖体RNA的动态变化及三维定位

Dynamics and three-dimensional localization of ribosomal RNA within the nucleolus.

作者信息

Thiry M, Cheutin T, O'Donohue M F, Kaplan H, Ploton D

机构信息

Laboratoire de Biologie Cellulaire et Tissulaire, Université de Liège, Belgique.

出版信息

RNA. 2000 Dec;6(12):1750-61. doi: 10.1017/s1355838200001564.

Abstract

Although rRNA synthesis, maturation, and assembly into preribosomal particles occur within the nucleolus, the route taken by pre-rRNAs from their synthetic sites toward the cytoplasm remains largely unexplored. Here, we employed a nondestructive method for the incorporation of BrUTP into the RNA of living cells. By using pulse-chase experiments, three-dimensional image reconstructions of confocal optical sections, and electron microscopy analysis of ultrathin sections, we were able to describe topological and spatial dynamics of rRNAs within the nucleolus. We identified the precise location and the volumic organization of four typical subdomains, in which rRNAs are successively moving towards the nucleolar periphery during their synthesis and processing steps. The incorporation of BrUTP takes place simultaneously within several tiny spheres, centered on the fibrillar centers. Then, the structures containing the newly synthesized RNAs enlarge and appear as compact ringlets disposed around the fibrillar centers. Later, they form hollow spheres surrounding the latter components and begin to fuse together. Finally, these structures widen and form large rings reaching the limits of the nucleoli. These results clearly show that the transport of pre-rRNAs within the nucleolus does not occur randomly, but appears as a radial flow starting from the fibrillar centers that form concentric rings, which finally fuse together as they progress toward the nucleolar periphery.

摘要

尽管核糖体RNA(rRNA)的合成、成熟以及组装成前核糖体颗粒的过程发生在核仁内,但前体rRNA从其合成位点向细胞质移动的途径在很大程度上仍未得到探索。在这里,我们采用了一种将5-溴尿苷三磷酸(BrUTP)掺入活细胞RNA的非破坏性方法。通过脉冲追踪实验、共聚焦光学切片的三维图像重建以及超薄切片的电子显微镜分析,我们能够描述核仁内rRNA的拓扑和空间动态。我们确定了四个典型亚结构域的精确位置和体积组织,在rRNA的合成和加工步骤中,它们依次向核仁周边移动。BrUTP的掺入同时发生在几个以纤维中心为中心的小球体内。然后,含有新合成RNA的结构扩大,并呈现为围绕纤维中心排列的紧密小环。随后,它们形成围绕后者成分的空心球体,并开始融合在一起。最后,这些结构变宽并形成到达核仁边缘的大环。这些结果清楚地表明,前体rRNA在核仁内的运输并非随机发生,而是表现为从形成同心环的纤维中心开始的径向流动,随着它们向核仁周边推进,最终融合在一起。

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