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The Candida albicans Lanosterol 14-α-Demethylase (ERG11) Gene Promoter Is Maximally Induced after Prolonged Growth with Antifungal Drugs

机译:抗真菌药长时间生长后最大程度地诱导了白色念珠菌羊毛甾醇14-α-脱甲基酶(ERG11)基因启动子。

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摘要

The azole antifungal drugs that target lanosterol 14-α-demethylase, encoded by the ERG11 gene, are used to treat a variety of infections caused by Candida albicans. Azoles are known to induce expression of ERG11 mRNA. The ERG11 promoter was cloned 5′ of the luciferase-coding region, and the induction of ERG11 expression by azoles was monitored by luciferase assays. Maximal induction of the ERG11 promoter by azoles occurs not during logarithmic growth but after the diauxic shift and requires azoles to be present throughout logarithmic growth. The effects of pH, carbon source, and aerobic or anaerobic growth on induction of the ERG11 promoter by azoles were analyzed. Treatment with terbinafine and fenpropimorph, which target other enzymes in the ergosterol biosynthetic pathway, also resulted in a delayed induction of ERG11 promoter activity. Nascent sterol synthesis was shown to parallel ERG11 promoter activity, and total sterols were reduced coincident with the timing of ERG11 promoter activation. These results as a whole suggest that expression of the ERG11 promoter is regulated in response to sterol depletion.
机译:由ERG11基因编码的靶向羊毛甾醇14-α-脱甲基酶的唑类抗真菌药用于治疗由白色念珠菌引起的多种感染。已知唑类可以诱导ERG11 mRNA的表达。将ERG11启动子克隆到荧光素酶编码区的5'端,并通过荧光素酶测定法监测由唑类诱导的ERG11表达。唑类化合物最大诱导ERG11启动子的过程不是在对数增长过程中,而是在双峰漂移之后,并且要求唑类化合物在整个对数增长过程中都存在。分析了pH,碳源,好氧或厌氧生长对唑类诱导ERG11启动子的影响。以麦角固醇生物合成途径中的其他酶为目标的特比萘芬和苯丙咪唑处理也导致ERG11启动子活性的诱导延迟。新生的甾醇合成显示出与ERG11启动子活性平行,并且总甾醇的减少与ERG11启动子激活的时间一致。总体上,这些结果表明,ERG11启动子的表达受固醇消耗的调节。

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