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Endocytosis in fission yeast is spatially associated with the actin cytoskeleton during polarised cell growth and cytokinesis

机译:在极化细胞生长和胞质分裂过程中,裂变酵母的内吞作用与肌动蛋白的细胞骨架在空间上相关

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In the fission yeast, Schizosaccharomyces pombe, uptake of the fluorescent styryl dye FM4-64 via the endocytic pathway to the vacuole was localised to the poles of growing, interphase cells and to the cell equator during cell division, regions of cell wall deposition that are rich in actin. When the pattern of growth or the plane of cytokinesis was altered, the relationship between the actin cytoskeleton and the site of endocytosis was maintained. Transfer of the label to the vacuolar membrane was dependent upon the Rab GTPase Ypt7 and, hence, vesicle fusion. Endocytic vesicles transiently colocalised with actin patches and endocytosis was inhibited in mutants that affected actin patch integrity and by the actin inhibitor latrunculin A. Concentrations of latrunculin that removed actin cables but left patches unaffected had no effect on endocytosis at the poles, but abolished endocytosis at the cell equator. Equatorial, but not polar, endocytosis was also inhibited in cells lacking the formin For3 (which have selectively destabilised actin cables), in mutants of the exocyst complex and in cells treated with brefeldin A. Differential effects on endocytosis at the cell poles and equator were also observed in the actin mutant cps8 and the Arp2/3 complex mutant arp2. The redirection of endocytosis from the cell poles to the cell equator in M phase coincided with the anaphase separation of sister chromatids and was abolished in the septation initiation network (SIN) mutants cdc7, sid1 and sid2, demonstrating that the spatial reorganisation of the endocytic pathway in the S. pombe cell cycle requires a functional SIN pathway. We conclude that endocytosis in fission yeast has two distinct components, both of which are actin-based, but which are mechanistically distinct, as well as being spatially and temporally separated in the S. pombe cell cycle.
机译:在裂殖酵母粟酒裂殖酵母中,荧光苯乙烯基染料FM4-64通过内吞途径进入液泡,位于细胞分裂过程中生长的两相细胞和细胞赤道的两极,即细胞壁沉积的区域。富含肌动蛋白。当生长方式或胞质分裂的平面改变时,肌动蛋白细胞骨架与内吞位点之间的关系得以维持。标记转移至液泡膜取决于Rab GTPase Ypt7,并因此取决于囊泡融合。在影响肌动蛋白斑完整性的突变体和肌动蛋白抑制剂latrunculin A中抑制了与肌动蛋白斑瞬时共处的内吞囊泡和内吞作用。肌动蛋白抑制剂latrunculin A抑制了latrunculin的浓度,去除了肌动蛋白索,但未受影响,对两极的内吞作用均无影响,但在细胞内吞噬作用被消除单元赤道。缺乏形式For3(具有选择性失稳的肌动蛋白电缆)的细胞,囊外复合体的突变体以及布雷菲德菌素A处理的细胞,也抑制了赤道的但不是极性的内吞作用。在细胞极和赤道上对内吞作用的差异是在肌动蛋白突变体cps8和Arp2 / 3复杂突变体arp2中也观察到。内吞作用在M期从细胞极向细胞赤道的重定向与姐妹染色单体的后期分离相吻合,并且在分隔起始网络(SIN)突变体cdc7,sid1和sid2中被取消,表明内吞途径的空间重组粟酒裂殖酵母细胞周期中的功能需要一个功能性SIN途径。我们得出的结论是,裂变酵母中的内吞作用具有两个不同的成分,这两个成分都是基于肌动蛋白的,但在机理上是不同的,并且在粟酒裂殖酵母细胞周期中在空间和时间上是分开的。

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