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γ-微管蛋白在中心体的募集及其微管核形成活性是由α-辅肌动蛋白引导的。

The centrosomal recruitment of γ-tubulin and its microtubule nucleation activity is α-fodrin guided.

机构信息

Cancer Research, Rajiv Gandhi Centre for Biotechnology, Thiruvananthapuram, India.

Department of Biotechnology, University of Kerala, Thiruvananthapuram, India.

出版信息

Cell Cycle. 2023 Feb;22(3):361-378. doi: 10.1080/15384101.2022.2119516. Epub 2022 Sep 9.

Abstract

The regulation and recruitment of γ-TuRCs, the prime nucleator of microtubules, to the centrosome are still thrust areas of research. The interaction of fodrin, a sub-plasmalemmal cytoskeletal protein, with γ-tubulin is a new area of interest. To understand the cellular significance of this interaction, we show that depletion of α-fodrin brings in a significant reduction of γ-tubulin in neural cell centrosomes making it functionally under-efficient. This causes a loss of nucleation ability that cannot efficiently form microtubules in interphase cells and astral microtubules in mitosis. Fluorescence Recovery after Photobleaching (FRAP) experiment implies that α-fodrin is important in the recruitment of γ-tubulin to the centrosome resulting in the aforementioned effects. Further, our experiments indicate that the interaction of α-fodrin with certain pericentriolar matrix proteins such as Pericentrin and CDK5RAP2 are crucial for the recruitment of γ-tubulin to the centrosome. Earlier we reported that α-fodrin limits the nucleation potential of γ-TuRC. In that context, this study suggests that α-fodrin is a γ-tubulin recruiting protein to the centrosome thus preventing cytoplasmic microtubule nucleation and thereby compartmentalizing the process to the centrosome for maximum efficiency. α-fodrin is a γ-tubulin interacting protein that controls the process of γ-tubulin recruitment to the centrosome and thereby regulates the microtubule nucleation capacity spatially and temporally.

摘要

γ-TuRC(微管的主要核形成物)向中心体的调节和募集仍然是研究的热点领域。 fodrin(质膜下细胞骨架蛋白)与γ-微管蛋白的相互作用是一个新的研究领域。为了了解这种相互作用的细胞意义,我们表明,α-fodrin 的耗竭会导致神经细胞中心体中 γ-微管蛋白的显著减少,从而使其功能效率降低。这导致核形成能力的丧失,无法在有丝分裂间期细胞和星体微管中有效地形成微管。荧光恢复后光漂白(FRAP)实验表明,α-fodrin 对于 γ-微管蛋白向中心体的募集很重要,从而导致了上述效应。此外,我们的实验表明,α-fodrin 与某些中心体周围基质蛋白(如 Pericentrin 和 CDK5RAP2)的相互作用对于 γ-微管蛋白向中心体的募集至关重要。此前我们报道过,α-fodrin 限制了 γ-TuRC 的核形成潜力。在这种情况下,本研究表明,α-fodrin 是一种向中心体募集 γ-微管蛋白的蛋白,从而防止细胞质微管核形成,并将该过程分区到中心体以实现最大效率。α-fodrin 是一种与 γ-微管蛋白相互作用的蛋白,控制 γ-微管蛋白向中心体的募集过程,从而在空间和时间上调节微管核形成能力。

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