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中心体蛋白CG-NAP和肯德林通过锚定γ-微管蛋白环复合物提供微管成核位点。

Centrosomal proteins CG-NAP and kendrin provide microtubule nucleation sites by anchoring gamma-tubulin ring complex.

作者信息

Takahashi Mikiko, Yamagiwa Akiko, Nishimura Tamako, Mukai Hideyuki, Ono Yoshitaka

机构信息

Biosignal Research Center, Kobe University, Japan.

出版信息

Mol Biol Cell. 2002 Sep;13(9):3235-45. doi: 10.1091/mbc.e02-02-0112.

Abstract

Microtubule assembly is initiated by the gamma-tubulin ring complex (gamma-TuRC). In yeast, the microtubule is nucleated from gamma-TuRC anchored to the amino-terminus of the spindle pole body component Spc110p, which interacts with calmodulin (Cmd1p) at the carboxy-terminus. However, mammalian protein that anchors gamma-TuRC remains to be elucidated. A giant coiled-coil protein, CG-NAP (centrosome and Golgi localized PKN-associated protein), was localized to the centrosome via the carboxyl-terminal region. This region was found to interact with calmodulin by yeast two-hybrid screening, and it shares high homology with the carboxyl-terminal region of another centrosomal coiled-coil protein, kendrin. The amino-terminal region of either CG-NAP or kendrin indirectly associated with gamma-tubulin through binding with gamma-tubulin complex protein 2 (GCP2) and/or GCP3. Furthermore, endogenous CG-NAP and kendrin were coimmunoprecipitated with each other and with endogenous GCP2 and gamma-tubulin, suggesting that CG-NAP and kendrin form complexes and interact with gamma-TuRC in vivo. These proteins were localized to the center of microtubule asters nucleated from isolated centrosomes. Pretreatment of the centrosomes by antibody to CG-NAP or kendrin moderately inhibited the microtubule nucleation; moreover, the combination of these antibodies resulted in stronger inhibition. These results imply that CG-NAP and kendrin provide sites for microtubule nucleation in the mammalian centrosome by anchoring gamma-TuRC.

摘要

微管组装由γ-微管蛋白环复合物(γ-TuRC)启动。在酵母中,微管从锚定在纺锤极体组分Spc110p氨基末端的γ-TuRC成核,Spc110p在羧基末端与钙调蛋白(Cmd1p)相互作用。然而,锚定γ-TuRC的哺乳动物蛋白仍有待阐明。一种巨大的卷曲螺旋蛋白,CG-NAP(中心体和高尔基体定位的PKN相关蛋白),通过羧基末端区域定位于中心体。通过酵母双杂交筛选发现该区域与钙调蛋白相互作用,并且它与另一种中心体卷曲螺旋蛋白kendrin的羧基末端区域具有高度同源性。CG-NAP或kendrin的氨基末端区域通过与γ-微管蛋白复合蛋白2(GCP2)和/或GCP3结合而间接与γ-微管蛋白相关联。此外,内源性CG-NAP和kendrin彼此以及与内源性GCP2和γ-微管蛋白共免疫沉淀,表明CG-NAP和kendrin形成复合物并在体内与γ-TuRC相互作用。这些蛋白定位于从分离的中心体成核的微管星状体的中心。用针对CG-NAP或kendrin的抗体对中心体进行预处理会适度抑制微管成核;此外,这些抗体的组合导致更强的抑制作用。这些结果表明,CG-NAP和kendrin通过锚定γ-TuRC为哺乳动物中心体中的微管成核提供位点。

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