首页> 外文期刊>Development >Cell-type-specific rescue of myosin function during Dictyostelium development defines two distinct cell movements required for culmination.
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Cell-type-specific rescue of myosin function during Dictyostelium development defines two distinct cell movements required for culmination.

机译:在网柄菌属发育过程中对肌球蛋白功能的细胞类型特异性拯救定义了达到顶点所需的两种不同的细胞运动。

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Mutant Dictyostelium cells lacking any of the component polypeptides of myosin II exhibit developmental defects. To define myosin's role in establishing Dictyostelium's developmental pattern, we have rescued myosin function in a myosin regulatory light chain null mutant (mlcR-) using cell-type-specific promoters. While mlcR- cells fail to progress beyond the mound stage, expression of RLC from the prestalk promoter, ecmA, produces culminants with normal stalks but with defects in spore cell localization. When GFP-marked prestalk and prespore cells expressing ecmA-RLC are mixed with wild-type cells, the mislocalization of prestalk cells, but not prespore cells, is rescued. Time-lapse video recording of ecmA-RLC cells showed that the posterior prespore zone failed to undergo a contraction important for the upward movement of prespore cells. Prespore cells marked with green fluorescent protein (GFP) failed to move toward the tip with the spiral motion typical of wild type. In contrast, expression of RLC in prespore cells using the psA promoter produced balloon-like structures reminiscent of sorocarps but lacking stalks. GFP-labeled prespore cells showed a spiral movement toward the top of the structures. Expression of RLC from the psA promoter restores the normal localization of psA-GFP cells, but not ecmA-GFP cells. These results define two distinct, myosin-dependent movements that are required for establishing a Dictyostelium fruiting body: stalk extension and active movement of the prespore zone that ensures proper placement of the spores atop the stalk. The approach used in these studies provides a direct means of testing the role of cell motility in distinct cell types during a morphogenetic program.
机译:缺乏肌球蛋白II的任何组成多肽的突变的单壁细胞显示出发育缺陷。为了定义肌球蛋白在建立盘基网柄菌的发育模式中的作用,我们使用细胞类型特异性启动子在肌球蛋白调节性轻链无效突变体(mlcR-)中拯救了肌球蛋白功能。尽管mlcR-细胞无法进展到堆肥阶段,但来自前茎启动子ecmA的RLC表达会产生具有正常茎的菌落,但孢子细胞定位存在缺陷。当将表达ecmA-RLC的GFP标记的前茎细胞和芽孢细胞与野生型细胞混合时,可以恢复前茎细胞而不是芽孢细胞的定位错误。 ecmA-RLC细胞的延时录像显示,后孢子区未能经历对于孢子细胞向上运动重要的收缩。带有绿色荧光蛋白(GFP)标记的孢子细胞未能以野生型的典型螺旋运动向尖端移动。相反,使用psA启动子在孢子前细胞中表达RLC产生的气球状结构让人联想起果皮,但缺乏茎。 GFP标记的孢子前细胞向结构顶部呈螺旋运动。来自psA启动子的RLC表达恢复了psA-GFP细胞的正常定位,但不能恢复ecmA-GFP细胞。这些结果定义了两个不同的,依赖肌球蛋白的运动,这些运动是建立Dictyostelium子实体所必需的:茎延伸和前孢子区的主动运动,以确保孢子在茎上的正确放置。这些研究中使用的方法提供了一种直接方法,可以在形态发生程序中测试细胞运动在不同细胞类型中的作用。

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