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液泡膜质子泵和质膜质子泵协同作用,以实现酵母细胞溶质pH稳态。

Vacuolar and plasma membrane proton pumps collaborate to achieve cytosolic pH homeostasis in yeast.

作者信息

Martínez-Muñoz Gloria A, Kane Patricia

机构信息

Department of Biochemistry and Molecular Biology, SUNY Upstate Medical University, Syracuse, NY 13210, USA.

出版信息

J Biol Chem. 2008 Jul 18;283(29):20309-19. doi: 10.1074/jbc.M710470200. Epub 2008 May 23.

Abstract

Vacuolar proton-translocating ATPases (V-ATPases) play a central role in organelle acidification in all eukaryotic cells. To address the role of the yeast V-ATPase in vacuolar and cytosolic pH homeostasis, ratiometric pH-sensitive fluorophores specific for the vacuole or cytosol were introduced into wild-type cells and vma mutants, which lack V-ATPase subunits. Transiently glucose-deprived wild-type cells respond to glucose addition with vacuolar acidification and cytosolic alkalinization, and subsequent addition of K(+) ion increases the pH of both the vacuole and cytosol. In contrast, glucose addition results in an increase in vacuolar pH in both vma mutants and wild-type cells treated with the V-ATPase inhibitor concanamycin A. Cytosolic pH homeostasis is also significantly perturbed in the vma mutants. Even at extracellular pH 5, conditions optimal for their growth, cytosolic pH was much lower, and response to glucose was smaller in the mutants. In plasma membrane fractions from the vma mutants, activity of the plasma membrane proton pump, Pma1p, was 65-75% lower than in fractions from wild-type cells. Immunofluorescence microscopy confirmed decreased levels of plasma membrane Pma1p and increased Pma1p at the vacuole and other compartments in the mutants. Pma1p was not mislocalized in concanamycin-treated cells, but a significant reduction in cytosolic pH under all conditions was still observed. We propose that short-term, V-ATPase activity is essential for both vacuolar acidification in response to glucose metabolism and for efficient cytosolic pH homeostasis, and long-term, V-ATPases are important for stable localization of Pma1p at the plasma membrane.

摘要

液泡质子转运ATP酶(V-ATP酶)在所有真核细胞的细胞器酸化过程中起着核心作用。为了研究酵母V-ATP酶在液泡和胞质pH稳态中的作用,将对液泡或胞质具有特异性的比率型pH敏感荧光团导入野生型细胞和缺乏V-ATP酶亚基的vma突变体中。短暂缺糖的野生型细胞在添加葡萄糖后会发生液泡酸化和胞质碱化,随后添加K(+)离子会使液泡和胞质的pH值都升高。相比之下,在vma突变体和用V-ATP酶抑制剂 concanamycin A处理的野生型细胞中,添加葡萄糖都会导致液泡pH值升高。vma突变体中的胞质pH稳态也受到显著干扰。即使在细胞外pH为5(对其生长最适宜的条件)时,突变体的胞质pH也低得多,且对葡萄糖的反应更小。在vma突变体的质膜组分中,质膜质子泵Pma1p的活性比野生型细胞组分中的低65-75%。免疫荧光显微镜检查证实,突变体中质膜Pma1p的水平降低,而液泡和其他区室中的Pma1p增加。Pma1p在concanamycin处理的细胞中没有发生错误定位,但在所有条件下仍观察到胞质pH显著降低。我们提出,短期而言,V-ATP酶活性对于响应葡萄糖代谢的液泡酸化和有效的胞质pH稳态都至关重要,长期而言,V-ATP酶对于Pma1p在质膜上的稳定定位很重要。

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