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Rvs161p and Sphingolipids Are Required for Actin Repolarization following Salt Stress

机译:盐胁迫后肌动蛋白复极化需要Rvs161p和鞘脂

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摘要

In Saccharomyces cerevisiae, the actin cytoskeleton is depolarized by NaCl stress. In this study, the response was maximal after 30 min, and then actin patches repolarized. Rvs161p was required for actin repolarization because the rvs161Δ mutant did not repolarize actin patches after growth in a salt medium. Mutations suppressing the rvs161Δ-related salt sensitivity all occurred in genes required for sphingolipid biosynthesis: FEN1, SUR4, SUR2, SUR1, and IPT1. These suppressors also suppressed act1-1-related salt sensitivity and the defect in actin repolarization of the rvs161Δ mutant, providing a link between sphingolipids and actin polarization. Indeed, deletion of the suppressor genes suppressed the rvs161Δ defect in actin repolarization in two ways: either actin was not depolarized at the wild-type level in a set of suppressor mutants, or actin was repolarized in the absence of Rvs161p in the other suppressor mutants. Rvs161p was localized as cortical patches that concentrated at polarization sites, i.e., bud emergence and septa, and was found to be associated with lipid rafts. An important link between sphingolipids and actin polarization is that Rvs161p was required for actin repolarization and was found to be located in lipid rafts.
机译:在酿酒酵母中,肌动蛋白的细胞骨架被NaCl胁迫去极化。在这项研究中,反应在30分钟后达到最大,然后肌动蛋白膜重新极化。肌动蛋白复极化需要Rvs161p,因为rvs161Δ突变体在盐培养基中生长后不会复极化肌动蛋白斑。抑制rvs161Δ相关盐敏感性的突变全部发生在鞘脂生物合成所需的基因中:FEN1,SUR4,SUR2,SUR1和IPT1。这些抑制剂还抑制了与act1-1相关的盐敏感性和rvs161Δ突变体的肌动蛋白复极化缺陷,从而在鞘脂和肌动蛋白极化之间建立了联系。实际上,删除抑制基因可通过两种方式抑制肌动蛋白复极化的rvs161Δ缺陷:要么在一组抑制突变体中肌动蛋白未在野生型水平去极化,要么在其他抑制突变体中在没有Rvs161p的情况下使肌动蛋白复极化。 。 Rvs161p被定位为集中在极化位点(即芽出芽和隔片)的皮质斑块,并被发现与脂质筏相关。鞘脂与肌动蛋白极化之间的重要联系是肌动蛋白重新极化需要Rvs161p,并且发现Rvs161p位于脂质筏中。

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