The position of the mitotic spindle determines the plane of cell cleavage, and thereby daughter cell location, size, and content. Spindle positioning is driven by dynein-mediated pulling forces exerted on astral microtubules, which requires an evolutionarily conserved complex of GαâGDP, GPR-1/2(Pins/LGN), and LIN-5(Mud/NuMA) proteins. To examine individual functions of the complex components, we developed a genetic strategy for light-controlled localization of endogenous proteins in C. elegans embryos. By replacing Gα and GPR-1/2 with a light-inducible membrane anchor, we demonstrate that GαâGDP, GαâGTP, and GPR-1/2 are not required for pulling-force generation. In the absence of Gα and GPR-1/2, cortical recruitment of LIN-5, but not dynein itself, induced high pulling forces. The light-controlled localization of LIN-5 overruled normal cell-cycle and polarity regulation and provided experimental control over the spindle and cell-cleavage plane. Our results define GαâGDP-GPR-1/2(Pins/LGN) as a regulatable membrane anchor, and LIN-5(Mud/NuMA) as a potent activator of dynein-dependent spindle-positioning forces.
Optogenetic dissection of mitotic spindle positioning in vivo.
利用光遗传学方法在体内解析有丝分裂纺锤体的定位
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作者:Fielmich Lars-Eric, Schmidt Ruben, Dickinson Daniel J, Goldstein Bob, Akhmanova Anna, van den Heuvel Sander
| 期刊: | Elife | 影响因子: | 6.400 |
| 时间: | 2018 | 起止号: | 2018 Aug 15; 7:e38198 |
| doi: | 10.7554/eLife.38198 | ||
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