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敲除高尔基体 Ca2+-ATP 酶 PMR1 基因增强了十二醇的抗真菌作用,该作用依赖于出芽酵母细胞内 Ca2+ 的积累。

Deletion of the Golgi Ca2+-ATPase PMR1 gene potentiates antifungal effects of dodecanol that depend on intracellular Ca2+ accumulation in budding yeast.

机构信息

Graduate School of Science, Osaka City University, Osaka, Japan.

Research Center for Urban Health and Sports, Osaka City University, Osaka, Japan.

出版信息

FEMS Yeast Res. 2020 Feb 1;20(1). doi: 10.1093/femsyr/foaa003.

DOI:10.1093/femsyr/foaa003
PMID:31942998
Abstract

One strategy for overcoming infectious diseases caused by drug-resistant fungi involves combining drugs rendered inactive by resistance with agents targeting the drug resistance mechanism. The antifungal activity of n-dodecanol disappears as incubation time passes. In Saccharomyces cerevisiae, anethole, a principal component of anise oil, prolongs the transient antifungal effect of dodecanol by downregulating genes of multidrug efflux pumps, mainly PDR5. However, the detailed mechanisms of dodecanol's antifungal action and the anethole-induced prolonged antifungal action of dodecanol are unknown. Screening of S. cerevisiae strains lacking genes related to Ca2+ homeostasis and signaling identified a pmr1Δ strain lacking Golgi Ca2+-ATPase as more sensitive to dodecanol than the parental strain. Dodecanol and the dodecanol + anethole combination significantly increased intracellular Ca2+ levels in both strains, but the mutant failed to clear intracellular Ca2+ accumulation. Further, dodecanol and the drug combination reduced PMR1 expression and did not lead to specific localization of Pmr1p in the parental strain after 4-h treatment. By contrast with the parental strain, dodecanol did not stimulate PDR5 expression in pmr1Δ. Based on these observations, we propose that the antifungal activity of dodecanol is related to intracellular Ca2+ accumulation, possibly dependent on PMR1 function, with anethole enabling Ca2+ accumulation by restricting dodecanol efflux.

摘要

克服耐药真菌引起的传染病的一种策略是将药物与针对耐药机制的药物结合使用。随着孵育时间的过去,正十二烷醇的抗真菌活性消失。在酿酒酵母中,茴脑,八角油的主要成分,通过下调多药外排泵基因,主要是 PDR5,延长了正十二烷醇的短暂抗真菌作用。然而,正十二烷醇的抗真菌作用的详细机制和茴脑诱导的正十二烷醇的延长抗真菌作用尚不清楚。筛选与 Ca2+ 稳态和信号转导相关基因缺失的酿酒酵母菌株,发现一种缺乏高尔基体 Ca2+-ATP 酶的 pmr1Δ 菌株比亲本菌株对正十二烷醇更敏感。正十二烷醇和正十二烷醇+茴脑组合在两种菌株中均显著增加细胞内 Ca2+水平,但突变体未能清除细胞内 Ca2+积累。此外,正十二烷醇和药物组合降低了 PMR1 的表达,并且在用 4 小时处理后,在亲本菌株中没有导致 Pmr1p 的特异性定位。与亲本菌株相比,pmr1Δ 中,正十二烷醇不能刺激 PDR5 的表达。基于这些观察,我们提出正十二烷醇的抗真菌活性与细胞内 Ca2+ 积累有关,可能依赖于 PMR1 功能,茴脑通过限制正十二烷醇外排来促进 Ca2+ 积累。

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