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首页> 外文期刊>The Journal of biological chemistry >Regulation of Vacuolar Proton-translocating ATPase Activity and Assembly by Extracellular pH
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Regulation of Vacuolar Proton-translocating ATPase Activity and Assembly by Extracellular pH

机译:通过细胞外pH调节真菌质子转移ATP酶活性和组装

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Vacuolar proton-translocating ATPases (V-ATPases) are responsible for organelle acidification in all eukaryotic cells. The yeast V-ATPase, known to be regulated by reversible disassembly in response to glucose deprivation, was recently reported to be regulated by extracellular pH as well (Padilla-López, S., and Pearce, D. A. (2006) J. Biol. Chem. 281, 10273–10280). Consistent with those results, we find 57% higher V-ATPase activity in vacuoles isolated after cell growth at extracellular pH of 7 than after growth at pH 5 in minimal medium. Remarkably, under these conditions, the V-ATPase also becomes largely insensitive to reversible disassembly, maintaining a low vacuolar pH and high levels of V1 subunit assembly, ATPase activity, and proton pumping during glucose deprivation. Cytosolic pH is constant under these conditions, indicating that the lack of reversible disassembly is not a response to altered cytosolic pH. We propose that when alternative mechanisms of vacuolar acidification are not available, maintaining V-ATPase activity becomes a priority, and the pump is not down-regulated in response to energy limitation. These results also suggest that integrated pH and metabolic inputs determine the final assembly state and activity of the V-ATPase.
机译:真空质子转移ATP酶(V-ATP酶)负责所有真核细胞中的细胞内酸化。最近据报道,酵母V-ATP酶,已知通过可逆拆卸响应于葡萄糖剥夺来调节术语,以通过细胞外pH调节(Padilla-lópez,S.和Pearce,Da(2006)J.Biol.Chem 。281,10273-10280)。与这些结果一致,我们发现在细胞生长在7的细胞间pH下的液泡中的57%较高的V-ATP酶活性比在最小培养基中pH 5的生长后的细胞生长。值得注意的是,在这些条件下,V-ATP酶也对可逆拆卸而大致不敏感,维持葡萄糖剥夺期间的低真空pH和高水平的V1亚基组件,ATP酶活性和质子泵送。在这些条件下,胞质pH是恒定的,表明缺乏可逆拆卸不是对改变的细胞溶质pH的反应。我们提出,当不可用的真空酸化的替代机制时,保持V-ATP酶活性成为优先级,并且泵响应于能量限制而不会下调。这些结果还表明,集成的pH和代谢输入确定了V-ATP酶的最终组装状态和活性。

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