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Polo样激酶是有丝分裂期间中心粒周围高尔基体堆栈碎片化所必需的。

Polo-like kinase is required for the fragmentation of pericentriolar Golgi stacks during mitosis.

作者信息

Sütterlin C, Lin C Y, Feng Y, Ferris D K, Erikson R L, Malhotra V

机构信息

Biology Department, University of California at San Diego, La Jolla, CA 92093, USA.

出版信息

Proc Natl Acad Sci U S A. 2001 Jul 31;98(16):9128-32. doi: 10.1073/pnas.161283998. Epub 2001 Jul 10.

Abstract

The pericentriolar stacks of Golgi cisternae undergo extensive reorganization during mitosis in mammalian cells. GM130 and GRASP65 (Golgi reassembly stacking protein of 65 kDa) are Golgi-associated proteins that are targets of mitotic kinases, and they have also been implicated in the reorganization of the Golgi structure during cell division. Previous studies have reported that mitogen-activated protein kinase kinase-1 (MEK1) and Cdc2 protein kinases are involved in these dynamic changes in the Golgi structure. More recently, the mitotic polo-like kinase (Plk) has been shown to interact with and phosphorylate GRASP65. Here, we provide evidence that Plk is involved in the mitosis-specific fragmentation of the Golgi apparatus. The addition of kinase-defective Plk or immunodepletion of Plk disrupts the fragmentation process. Furthermore, Golgi fragmentation is inhibited by the addition of either full-length or truncated GRASP65. These findings suggest that phosphorylation of GRASP65 by Plk may be a critical event in the reorganization of the Golgi structure during mitosis.

摘要

在哺乳动物细胞有丝分裂过程中,高尔基体囊泡的中心粒周围堆叠会经历广泛的重组。GM130和GRASP65(65 kDa的高尔基体重新组装堆叠蛋白)是与高尔基体相关的蛋白质,它们是有丝分裂激酶的作用靶点,并且在细胞分裂过程中也与高尔基体结构的重组有关。先前的研究报道,丝裂原活化蛋白激酶激酶-1(MEK1)和Cdc2蛋白激酶参与了高尔基体结构的这些动态变化。最近,有丝分裂的polo样激酶(Plk)已被证明与GRASP65相互作用并使其磷酸化。在此,我们提供证据表明Plk参与了高尔基体在有丝分裂特异性的碎片化过程。添加激酶缺陷型Plk或对Plk进行免疫去除会破坏碎片化过程。此外,添加全长或截短的GRASP65均可抑制高尔基体碎片化。这些发现表明,Plk对GRASP65的磷酸化可能是有丝分裂期间高尔基体结构重组中的一个关键事件。

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