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通过绿色荧光蛋白-钙调蛋白融合蛋白技术揭示的HeLa细胞在细胞分裂过程中钙调蛋白的动态重新分布。

Dynamic redistribution of calmodulin in HeLa cells during cell division as revealed by a GFP-calmodulin fusion protein technique.

作者信息

Li C J, Heim R, Lu P, Pu Y, Tsien R Y, Chang D C

机构信息

Department of Biology, Hong Kong University of Science and Technology, Clear Water Bay, Hong Kong.

出版信息

J Cell Sci. 1999 May;112 ( Pt 10):1567-77. doi: 10.1242/jcs.112.10.1567.

DOI:10.1242/jcs.112.10.1567
PMID:10212150
Abstract

It has been suggested by many studies that Ca2+ signaling plays an important role in regulating key steps in cell division. In order to study the down stream components of calcium signaling, we have fused the gene of calmodulin (CaM) with that of green fluorescent protein (GFP) and expressed it in HeLa cells. The GFP-CaM protein was found to have similar biochemical properties as the wild-type CaM, and its distribution was also similar to that of the endogenous CaM. Using this GFP-tagged CaM as a probe, we have conducted a detailed examination of the spatial- and temporal-dependent redistribution of calmodulin in living mammalian cells during cell division. Our major findings are: (1) high density of CaM was found to distribute in two sub-cellular locations during mitosis; one fraction was concentrated in the spindle poles, while the other was concentrated in the sub-membrane region around the cell. (2) The sub-membrane fraction of CaM became aggregated at the equatorial region where the cleavage furrow was about to form. The timing of this localized aggregation of CaM was closely associated with the onset of cytokinesis. (3) Using a TA-CaM probe, we found that the sub-membrane fraction of CaM near the cleavage furrow was selectively activated during cell division. (4) When we injected a CaM-specific inhibitory peptide into early anaphase cells, cytokinesis was either blocked or severely delayed. These findings suggest that, in addition to Ca2+ ion, CaM may represent a second signal that can also play an active role in determining the positioning and timing of the cleavage furrow formation.

摘要

许多研究表明,Ca2+信号在调节细胞分裂的关键步骤中起着重要作用。为了研究钙信号的下游成分,我们将钙调蛋白(CaM)基因与绿色荧光蛋白(GFP)基因融合,并在HeLa细胞中表达。发现GFP-CaM蛋白具有与野生型CaM相似的生化特性,其分布也与内源性CaM相似。利用这种GFP标记的CaM作为探针,我们对活的哺乳动物细胞在细胞分裂过程中钙调蛋白的时空依赖性重新分布进行了详细研究。我们的主要发现如下:(1)在有丝分裂期间,发现高密度的CaM分布在两个亚细胞位置;一部分集中在纺锤体极,而另一部分集中在细胞周围的亚膜区域。(2)CaM的亚膜部分在即将形成分裂沟的赤道区域聚集。CaM这种局部聚集的时间与胞质分裂的开始密切相关。(3)使用TA-CaM探针,我们发现在细胞分裂期间,靠近分裂沟的CaM亚膜部分被选择性激活。(4)当我们向后期早期细胞注射CaM特异性抑制肽时,胞质分裂要么被阻断,要么严重延迟。这些发现表明,除了Ca2+离子外,CaM可能代表第二种信号,在决定分裂沟形成的位置和时间方面也可能发挥积极作用。

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