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中心体分离:微管和肌动蛋白丝的各自作用

Centrosome separation: respective role of microtubules and actin filaments.

作者信息

Uzbekov Rustem, Kireyev Igor, Prigent Claude

机构信息

Groupe cycle cellulaire, UMR 6061 génétique et développement, CNRS-Université de Rennes 1, IFR 97 génomique et santé Faculté de médecine, 2, avenue du Professeur Léon Bernard, CS 34317, 35043 Rennes cedex, France.

出版信息

Biol Cell. 2002 Sep;94(4-5):275-88. doi: 10.1016/s0248-4900(02)01202-9.

DOI:10.1016/s0248-4900(02)01202-9
PMID:12489696
Abstract

In mammalian cells, the separation of centrosomes is a prerequisite for bipolar mitotic spindle assembly. We have investigated the respective contribution of the two cytoskeleton components, microtubules and actin filaments, in this process. Distances between centrosomes have been measured during cell cycle progression in Xenopus laevis XL2 cultured cells in the presence or absence of either network. We considered two stages in centrosome separation: the splitting stage, when centrosomes start to move apart (minimum distance of 1 microm), and the elongation stage (from 1 to 7 microm). In interphase, depolymerisation of microtubules by nocodazole significantly inhibited the splitting stage, while the elongation stage was, on the contrary, facilitated. In mitosis, while nocodazole treatment completely blocked spindle assembly, in prophase, we observed that 55% of the centrosomes separated, versus 94% in the control. Upon actin depolymerisation by latrunculin, splitting of the interphase centrosome was blocked, and cells entered mitosis with unseparated centrosomes. Cells compensated for this separation delay by increasing the length of both prophase and prometaphase stages to allow for centrosome separation until a minimal distance was reached. Then the cells passed through anaphase, performing proper chromosome separation, but cytokinesis did not occur, and binuclear cells were formed. Our results clearly show that the actin microfilaments participate in centrosome separation at the G2/M transition and work in synergy with the microtubules to accelerate centrosome separation during mitosis.

摘要

在哺乳动物细胞中,中心体的分离是双极有丝分裂纺锤体组装的前提条件。我们研究了细胞骨架的两个组成部分,即微管和肌动蛋白丝,在此过程中的各自作用。在非洲爪蟾XL2培养细胞的细胞周期进程中,在有或无任何一种网络存在的情况下,测量了中心体之间的距离。我们考虑了中心体分离的两个阶段:分裂阶段,即中心体开始分开移动时(最小距离为1微米),以及伸长阶段(从1到7微米)。在间期,诺考达唑使微管解聚显著抑制了分裂阶段,而伸长阶段则相反,得到了促进。在有丝分裂中,虽然诺考达唑处理完全阻断了纺锤体组装,但在前期,我们观察到55%的中心体分离,而对照组为94%。用拉春库林使肌动蛋白解聚后,间期中心体的分裂被阻断,细胞进入有丝分裂时中心体未分离。细胞通过延长前期和前中期的长度来弥补这种分离延迟,以允许中心体分离,直到达到最小距离。然后细胞进入后期,进行正常的染色体分离,但胞质分裂未发生,形成了双核细胞。我们的结果清楚地表明,肌动蛋白微丝在G2/M转换时参与中心体分离,并与微管协同作用,在有丝分裂期间加速中心体分离。

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