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Potassium deprivation is sufficient to induce a cell death program in Saccharomyces cerevisiae

机译:缺钾足以诱导酿酒酵母中的细胞死亡程序

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Cell culture in low potassium (K) media has been associated to programmed cell death (PCD) in metazoans. In this study, deprivation of K led Saccharomyces cerevisiae cells to a death process that involved phosphatidylserine externalization, changes in chromatin condensation, DNA and vacuole fragmentation as well as enhanced accumulation of reactive oxygen species. During the course of K starvation, plasma membrane hyperpolarization and increased accumulation of calcium (Capo) took place. The presence of rubidium (Rb), a K-analogue element, in the K-deprived medium was accompanied by Rb accumulation but did not fully prevent the appearance of PCD markers. This argues for a specific effect of K on the course of cell death. While the absence of the YCA1 metacaspase did not have a major effect, the absence of TRK (transport of K) K-transporters led to changes in the pattern of annexin V/propidium iodide labeling. This change paralleled a fast accumulation of Capo. Addition of ethylene glycol tetraacetic acid improved growth and reduced cell death in trk1trk2 cells. These findings reveal that K deprivation is sufficient to induce PCD in a cell-walled eukaryotic organism and suggest that the phenotype attributed to the lack of TRK genes is partially due to the effect of the encoded transporters on Capo homeostasis.
机译:低钾(K)培养基中的细胞培养与后生动物的程序性细胞死亡(PCD)相关。在这项研究中,K的缺乏导致酿酒酵母细胞死亡,其过程涉及磷脂酰丝氨酸的外在化,染色质缩合的改变,DNA和液泡的碎片化以及活性氧的积累。在缺钾的过程中,发生了质膜超极化和钙积累(Capo)增加。缺钾培养基中存在-类似元素rub(Rb),但伴随Rb积累,但并未完全阻止PCD标记物的出现。这证明了K对细胞死亡过程的特定作用。虽然缺少YCA1 metaaspase不会产生重大影响,但缺少TRK(钾的转运)K-转运蛋白会导致膜联蛋白V /碘化丙啶标记的模式发生变化。这种变化与Capo的快速积累并存。乙二醇四乙酸的添加改善了trk1trk2细胞的生长并降低了细胞死亡。这些发现表明,剥夺钾足以诱导细胞壁真核生物中的PCD,并表明归因于TRK基因缺乏的表型部分是由于编码的转运蛋白对Capo稳态的影响。

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