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酿酒酵母高渗透压甘油和细胞壁完整性丝裂原活化蛋白激酶途径参与适应细胞毒素 HM-1 的作用。

The high-osmolarity glycerol- and cell wall integrity-MAP kinase pathways of Saccharomyces cerevisiae are involved in adaptation to the action of killer toxin HM-1.

机构信息

Department of Biochemistry, Faculty of Pharmaceutical Sciences, Niigata University of Pharmacy and Applied Life Sciences, Niigata, Japan.

出版信息

Yeast. 2012 Nov;29(11):475-85. doi: 10.1002/yea.2927. Epub 2012 Oct 15.

DOI:10.1002/yea.2927
PMID:23065846
Abstract

Fps1p is an aquaglyceroporin important for turgor regulation of Saccharomyces cerevisiae. Previously we reported the involvement of Fps1p in the yeast-killing action of killer toxin HM-1. The fps1 cells showed a high HM-1-resistant phenotype in hypotonic medium and an HM-1-susceptible phenotype in hypertonic medium. This osmotic dependency in HM-1 susceptibility was similar to those observed in Congo red, but different from those observed in other cell wall-disturbing agents. These results indicate that HM-1 exerts fungicidal activity mainly by binding and inserting into the yeast cell wall structure, rather than by inhibiting 1,3-β-glucan synthase. We next determined HM-1-susceptibility and diphospho-MAP kinase inductions in S. cerevisiae. In the wild-type cell, expressions of diphospho-Hog1p and -Slt2p, and mRNA transcription of CWP1 and HOR2, were induced within 1 h after an addition of HM-1. ssk1 and pbs2 cells, but not sho1 and hkr1 cells, showed HM-1-sensitive phenotypes and lacked inductions of phospho-Hog1p in response to HM-1. mid2, rom2 and bck1 cells showed HM-1-sensitive phenotypes and decreased inductions of phospho-Slt2p in response to HM-1. From these results, we postulated that the Sln1-Ypd1-Ssk1 branch of the high-osmolality glycerol (HOG) pathway and plasma membrane sensors of the cell wall integrity (CWI) pathway detect cell wall stresses caused by HM-1. We further suggested that activations of both HOG and CWI pathways have an important role in the adaptive response to HM-1 toxicity.

摘要

Fps1p 是一种水甘油通道蛋白,对酿酒酵母的渗透压调节很重要。之前我们报道过 Fps1p 参与了杀伤性毒素 HM-1 的酵母杀伤作用。在低渗培养基中,fps1 细胞表现出对 HM-1 的高抗性表型,而在高渗培养基中表现出对 HM-1 的敏感性表型。这种对 HM-1 敏感性的渗透压依赖性与刚果红观察到的相似,但与其他细胞壁干扰剂观察到的不同。这些结果表明,HM-1 主要通过结合并插入酵母细胞壁结构来发挥杀菌活性,而不是通过抑制 1,3-β-葡聚糖合酶。我们接下来确定了 S. cerevisiae 对 HM-1 的敏感性和双磷酸化-MAP 激酶的诱导。在野生型细胞中,在添加 HM-1 后 1 小时内,双磷酸化-Hog1p 和 -Slt2p 的表达以及 CWP1 和 HOR2 的 mRNA 转录被诱导。ssk1 和 pbs2 细胞,但不是 sho1 和 hkr1 细胞,表现出对 HM-1 的敏感性表型,并且对 HM-1 没有诱导磷酸化-Hog1p 的表达。mid2、rom2 和 bck1 细胞表现出对 HM-1 的敏感性表型,并且对 HM-1 的诱导磷酸化-Slt2p 的表达减少。根据这些结果,我们假设高渗透压甘油(HOG)途径的 Sln1-Ypd1-Ssk1 分支和细胞壁完整性(CWI)途径的质膜传感器检测 HM-1 引起的细胞壁应激。我们进一步提出,HOG 和 CWI 途径的激活在适应 HM-1 毒性的过程中起着重要作用。

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