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通过特定半胱氨酸残基的谷胱甘肽化来调节酵母电压门控 Ca 通道同源物 Cch1p 的氧化还原状态。

Redox regulation of the yeast voltage-gated Ca channel homolog Cch1p by glutathionylation of specific cysteine residues.

机构信息

Department of Biological Sciences, Indian Institute of Science Education & Research (IISER), Sector 81, Mohali, Punjab 140306, India.

Department of Biological Sciences, Indian Institute of Science Education & Research (IISER), Sector 81, Mohali, Punjab 140306, India

出版信息

J Cell Sci. 2017 Jul 15;130(14):2317-2328. doi: 10.1242/jcs.202853. Epub 2017 Jun 2.

DOI:10.1242/jcs.202853
PMID:28576969
Abstract

Cch1p, the yeast homolog of the pore-forming subunit α of the mammalian voltage-gated Ca channel (VGCC), is located on the plasma membrane and mediates the redox-dependent influx of Ca Cch1p is known to undergo both rapid activation (after oxidative stress and or a change to high pH) and slow activation (after ER stress and mating pheromone activation), but the mechanism of activation is not known. We demonstrate here that both the fast activation (exposure to pH 8-8.5 or treatment with HO) and the slow activation (treatment with tunicamycin or α-factor) are mediated through a common redox-dependent mechanism. Furthermore, through mutational analysis of all 18 exposed cysteine residues in the Cch1p protein, we show that the four mutants C587A, C606A, C636A and C642A, which are clustered together in a common cytoplasmic loop region, were functionally defective for both fast and slow activations, and also showed reduced glutathionylation. These four cysteine residues are also conserved across phyla, suggesting a conserved mechanism of activation. Investigations into the enzymes involved in the activation reveal that the yeast glutathione S-transferase Gtt1p is involved in the glutathionylation of Cch1p, while the thioredoxin Trx2p plays a role in the Cch1p deglutathionylation.

摘要

酵母电压门控钙通道(VGCC)形成亚单位α的同源物 Cch1p 位于质膜上,介导氧化还原依赖性钙内流。已知 Cch1p 既可以快速激活(在氧化应激或 pH 值升高后),也可以缓慢激活(在 ER 应激和交配信息素激活后),但激活机制尚不清楚。我们在这里证明,快速激活(暴露于 pH8-8.5 或用 HO 处理)和缓慢激活(用衣霉素或α-因子处理)都是通过共同的氧化还原依赖机制介导的。此外,通过对 Cch1p 蛋白中所有 18 个暴露半胱氨酸残基的突变分析,我们发现四个突变体 C587A、C606A、C636A 和 C642A,它们聚集在一个共同的细胞质环区域,在快速和缓慢激活中均功能缺陷,并且还显示出谷胱甘肽化减少。这四个半胱氨酸残基在所有门中都是保守的,这表明存在一种保守的激活机制。对参与激活的酶的研究表明,酵母谷胱甘肽 S-转移酶 Gtt1p 参与 Cch1p 的谷胱甘肽化,而硫氧还蛋白 Trx2p 在 Cch1p 的去谷胱甘肽化中发挥作用。

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