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非肌肉肌球蛋白 IIA 和 IIB 对人永生化成纤维细胞胞质分裂的差异贡献。

Differential contributions of nonmuscle myosin IIA and IIB to cytokinesis in human immortalized fibroblasts.

机构信息

Graduate School of Chemical Sciences and Engineering, Hokkaido University, Sapporo 060-8628, Japan.

Research Institute for Electronic Science, Hokkaido University, Sapporo 001-0020, Japan.

出版信息

Exp Cell Res. 2019 Mar 1;376(1):67-76. doi: 10.1016/j.yexcr.2019.01.020. Epub 2019 Jan 31.

Abstract

Nonmuscle myosin II (NMII) plays an important role in cytokinesis by constricting a contractile ring. However, it is poorly understood how NMII isoforms contribute to cytokinesis in mammalian cells. Here, we investigated the roles of the two major NMII isoforms, NMIIA and NMIIB, in cytokinesis using a WI-38 VA13 cell line (human immortalized fibroblast). In this cell line, NMIIB tended to localize to the contractile ring more than NMIIA. The expression level of NMIIA affected the localization of NMIIB. Most NMIIB accumulated at the cleavage furrow in NMIIA-knockout (KO) cells, and most NMIIA was displaced from this location in exogenous NMIIB-expressing cells, indicating that NMIIB preferentially localizes to the contractile ring. Specific KO of each isoform elicited opposite effects. The rate of furrow ingression was decreased and increased in NMIIA-KO and NMIIB-KO cells, respectively. Meanwhile, the length of NMII-filament stacks in the contractile ring was increased and decreased in NMIIA-KO and NMIIB-KO cells, respectively. Moreover, NMIIA helped to maintain cortical stiffness during cytokinesis. These findings suggest that appropriate ratio of NMIIA and NMIIB in the contractile ring is important for proper cytokinesis in specific cell types. In addition, two-photon excitation spinning-disk confocal microscopy enabled us to image constriction of the contractile ring in live cells in a three-dimensional manner.

摘要

非肌肉肌球蛋白 II(NMII)通过收缩收缩环在胞质分裂中发挥重要作用。然而,NMII 同工型如何有助于哺乳动物细胞的胞质分裂仍知之甚少。在这里,我们使用 WI-38 VA13 细胞系(人永生化成纤维细胞)研究了两种主要的 NMII 同工型 NMIIA 和 NMIIB 在胞质分裂中的作用。在该细胞系中,NMIIB 比 NMIIA 更倾向于定位到收缩环。NMIIA 的表达水平影响 NMIIB 的定位。NMIIA 敲除(KO)细胞中 NMIIB 大量积累在分裂沟处,外源性 NMIIB 表达细胞中 NMIIA 大部分被置换出该位置,表明 NMIIB 优先定位到收缩环。每种同工型的特异性 KO 引起相反的效果。在 NMIIA-KO 和 NMIIB-KO 细胞中,沟的侵入率分别降低和增加。同时,在 NMIIA-KO 和 NMIIB-KO 细胞中,收缩环中 NMII 纤维堆的长度分别增加和减少。此外,NMIIA 在胞质分裂过程中有助于维持皮质硬度。这些发现表明,收缩环中 NMIIA 和 NMIIB 的适当比例对于特定细胞类型的正常胞质分裂是重要的。此外,双光子激发旋转盘共聚焦显微镜使我们能够以三维方式对活细胞中收缩环的收缩进行成像。

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