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粟酒裂殖酵母ehs1p参与维持细胞壁完整性和钙摄取。

Schizosaccharomyces pombe ehs1p is involved in maintaining cell wall integrity and in calcium uptake.

作者信息

Carnero E, Ribas J C, García B, Durán A, Sánchez Y

机构信息

Departamento de Microbiología y Genética, Instituto de Microbiología Bioquímica, CSIC and Universidad de Salamanca, Spain.

出版信息

Mol Gen Genet. 2000 Sep;264(1-2):173-83. doi: 10.1007/s004380000318.

DOI:10.1007/s004380000318
PMID:11016847
Abstract

The Schizosaccharomyces pombe mutant ehs1-1 mutant was isolated on the basis of its hypersensitivity to Echinocandin and Calcofluor White, which inhibit cell wall synthesis. The mutant shows a thermosensitive growth phenotype that is suppressed in the presence of an osmotic stabiliser. The mutant also showed other cell wall-associated phenotypes, such as enhanced sensitivity to enzymatic cell wall degradation and an imbalance in polysaccharide synthesis. The ehs1 + gene encodes a predicted integral membrane protein that is 30% identical to Saccharomyces cerevisiae Mid1p, a protein that has been proposed to form part of a calcium channel. As expected for such a function, we found that ehs1+ is involved in intracellular Ca2+ accumulation. High external Ca2+ concentrations suppressed all phenotypes associated with the ehs1 null mutation, suggesting that the cell integrity defects of ehs1 mutants result from inadequate levels of calcium in the cell. We observed a genetic relationship between ehs1+ and the protein kinase C homologue pck2+. pck2+ suppressed all phenotypes of ehs1-1 mutant cells. Overproduction of pck2p is deleterious to wild-type cells, increasing 1,3-beta-D-glucan synthase activity and promoting accumulation of extremely high levels of Ca2+. The lethality associated with pck2p, the increase in 1,3-beta-D-glucan synthase production and the strong Ca2+ accumulation are all dependent on the presence of ehs1p. Our results suggest that in fission yeast ehs1p forms part of a calcium channel that is involved in the cell wall integrity pathway that includes the kinase pck2p.

摘要

粟酒裂殖酵母突变体ehs1-1是基于其对抑制细胞壁合成的棘白菌素和荧光增白剂高度敏感而分离得到的。该突变体表现出温度敏感型生长表型,在存在渗透稳定剂的情况下这种表型受到抑制。该突变体还表现出其他与细胞壁相关的表型,如对酶促细胞壁降解的敏感性增强以及多糖合成失衡。ehs1+基因编码一种预测的整合膜蛋白,与酿酒酵母的Mid1p有30%的同源性,Mid1p被认为是钙通道的一部分。正如预期的这种功能一样,我们发现ehs1+参与细胞内Ca2+的积累。高浓度的外部Ca2+抑制了与ehs1基因缺失突变相关的所有表型,这表明ehs1突变体的细胞完整性缺陷是由于细胞内钙水平不足所致。我们观察到ehs1+与蛋白激酶C同源物pck2+之间存在遗传关系。pck2+抑制了ehs1-1突变体细胞的所有表型。pck2p的过量表达对野生型细胞有害,会增加1,3-β-D-葡聚糖合酶的活性并促进极高水平Ca2+的积累。与pck2p相关的致死性、1,3-β-D-葡聚糖合酶产量的增加以及强烈的Ca2+积累都依赖于ehs1p的存在。我们的结果表明,在裂殖酵母中,ehs1p是钙通道的一部分,该通道参与包括激酶pck2p在内的细胞壁完整性途径。

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