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The Dynamic Pollen Tube Cytoskeleton: Live Cell Studies Using Actin-Binding and Microtubule-Binding Reporter Proteins

机译:动态花粉管细胞骨架:使用肌动蛋白结合和微管结合记者蛋白的活细胞研究。

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Pollen tubes elongate within the pistil to transport sperm cells to the embryo sac for fertilization. Growth occurs exclusively at the tube apex, rendering pollen tube elongation a most dramatic polar cell growth process. A hallmark pollen tube feature is its cytoskeleton, which comprises elaborately organized and dynamic actin microfilaments and microtubules. Pollen tube growth is dependent on the actin cytoskeleton; its organization and regulation have been examined extensively by various approaches, including fluorescent protein labeled actin-binding proteins in live cell studies. Using the previously described GFP-NtADF1 and GFP-LlADF1, and a new actin reporter protein NtPLIM2b-GFP, we re-affirm that the predominant actin structures in elongating tobacco and lily pollen tubes are long, streaming actin cables along the pollen tube shank, and a subapical structure comprising shorter actin cables. The subapical collection of actin microfilaments undergoes dynamic changes, giving rise to the appearance of structures that range from basket- or funnel-shaped, mesh-like to a subtle ring. NtPLIM2b-GFP is used in combination with a guanine nucleotide exchange factor for the Rho GTPases, AtROP-GEF1, to illustrate the use of these actin reporter proteins to explore the linkage between the polar cell growth process and its actin cytoskeleton. Contrary to the actin cytoskeleton, microtubules appear not to play a direct role in supporting the polar cell growth process in angiosperm pollen tubes. Using a microtubule reporter protein based on the microtubule end-binding protein from Arabidopsis AtEB1, GFP-AtEB1, we show that the extensive microtubule network in elongating pollen tubes displays varying degrees of dynamics. These reporter proteins provide versatile tools to explore the functional connection between major structural and signaling components of the polar pollen tube growth process.
机译:花粉管在雌蕊内伸长,将精子细胞转运至胚囊进行受精。生长仅发生在管尖,使花粉管伸长成为最引人注目的极性细胞生长过程。花粉管的标志性特征是其细胞骨架,其中包括精心组织和动态的肌动蛋白微丝和微管。花粉管的生长取​​决于肌动蛋白的细胞骨架。它的组织和调节已通过各种方法进行了广泛研究,包括在活细胞研究中用荧光蛋白标记的肌动蛋白结合蛋白。使用先前描述的GFP-NtADF1和GFP-LlADF1,以及新的肌动蛋白报道蛋白NtPLIM2b-GFP,我们再次确认伸长的烟草和百合花粉管中的主要肌动蛋白结构是长的,沿着花粉管柄流动的肌动蛋白电缆,以及包含较短的肌动蛋白电缆的根尖下结构。肌动蛋白微丝的根尖下发生动态变化,从而出现从篮状或漏斗状,网状到细微环的结构外观。 NtPLIM2b-GFP与鸟嘌呤核苷酸交换因子一起用于Rho GTPases AtROP-GEF1,以说明这些肌动蛋白报道蛋白在极地细胞生长过程及其肌动蛋白细胞骨架之间的联系。与肌动蛋白的细胞骨架相反,微管似乎在支持被子植物花粉管中的极性细胞生长过程中不发挥直接作用。使用基于来自拟南芥AtEB1,GFP-AtEB1的微管末端结合蛋白的微管报道蛋白,我们显示在延长的花粉管中广泛的微管网络显示不同程度的动力学。这些报告蛋白提供了多种工具,可探索极性花粉管生长过程的主要结构和信号成分之间的功能联系。

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  • 来源
    《Molecular Plant》 |2008年第4期|p.686-702|共17页
  • 作者单位

    aDepartment of Biochemistry and Molecular Biology bMolecular Cell Biology Program cPlant Biology Graduate Program, University of Massachusetts, Lederle Graduate Research Tower, Amherst, MA 01003, USA dInstituto Gulbenkian de Ciencia, Centro de Biologia de Desenvolvimento, PT-2780–156 Oeiras, Portugal eUniversidale de Lisboa, Faculdade de Ciencias, Dept. Biologia Vegetal, Campo Grande, Ed.C2. PT-1749–016 Lisboa, Portugal fPresent address: School of Biosciences, University of Birmingham, Edgbaston B15 2TT, UK gPresent address: Department of Biology, University of Washington, Box 351800, Seattle, WA 98195, USA;

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