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锌状态和液泡锌转运蛋白控制酿酒酵母中碱性磷酸酶的积累和活性。

Zinc status and vacuolar zinc transporters control alkaline phosphatase accumulation and activity in Saccharomyces cerevisiae.

作者信息

Qiao Wei, Ellis Charissa, Steffen Janet, Wu Chang-Yi, Eide David J

机构信息

Department of Nutritional Sciences, University of Wisconsin-Madison, Madison, WI 53706, USA.

出版信息

Mol Microbiol. 2009 Apr;72(2):320-34. doi: 10.1111/j.1365-2958.2009.06644.x. Epub 2009 Mar 3.

Abstract

Little is known about how metalloproteins in the secretory pathway obtain their metal ion cofactors. We used the Pho8 alkaline phosphatase of the yeast Saccharomyces cerevisiae to probe this process in vivo. We found that both Pho8 activity and protein accumulation are zinc-dependent and decrease in zinc-limited cells. Low Pho8 accumulation was the result of degradation by vacuolar proteases. Surprisingly, the protective effect of zinc on Pho8 stability was not solely due to Zn(2+) binding to the active-site ligands suggesting that the Pho8 protein is targeted for degradation in zinc-limited cells by another mechanism. Pho8 appears to be a rare example of a metalloprotein whose stability is regulated by its metal cofactor independently of active-site binding. We also assessed which zinc transporters are responsible for supplying zinc to Pho8. We found that the Zrc1 and Cot1 vacuolar zinc transporters play the major role while the Msc2/Zrg17 zinc transporter complex active in the endoplasmic reticulum is not involved. These results demonstrate that the vacuolar zinc transporters, previously implicated in metal detoxification, also deliver zinc to certain metalloproteins within intracellular compartments. These data suggest that Pho8 receives its metal cofactor in the vacuole rather than in earlier compartments of the secretory pathway.

摘要

关于分泌途径中的金属蛋白如何获得其金属离子辅因子,人们了解甚少。我们利用酿酒酵母的Pho8碱性磷酸酶在体内探究这一过程。我们发现Pho8活性和蛋白积累均依赖于锌,且在锌限制的细胞中会降低。Pho8积累量低是液泡蛋白酶降解的结果。令人惊讶的是,锌对Pho8稳定性的保护作用并非仅仅归因于Zn(2+)与活性位点配体的结合,这表明Pho8蛋白在锌限制的细胞中是通过另一种机制被靶向降解的。Pho8似乎是一种罕见的金属蛋白例子,其稳定性由金属辅因子独立于活性位点结合来调节。我们还评估了哪些锌转运蛋白负责为Pho8供应锌。我们发现Zrc1和Cot1液泡锌转运蛋白起主要作用,而在内质网中活跃的Msc2/Zrg17锌转运蛋白复合物则不涉及。这些结果表明,先前与金属解毒有关的液泡锌转运蛋白,也会将锌递送至细胞内区室中的某些金属蛋白。这些数据表明Pho8在液泡中而非分泌途径的早期区室中获得其金属辅因子。

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