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Overexpression or Deletion of Ergosterol Biosynthesis Genes Alters Doubling Time, Response to Stress Agents, and Drug Susceptibility in Saccharomyces cerevisiae

机译:麦芽固醇生物合成基因的过表达或缺失改变了酿酒酵母的倍增时间,对应激源的反应以及药物敏感性

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ABSTRACT Ergosterol (ERG) is a critical sterol in the cell membranes of fungi, and its biosynthesis is tightly regulated by 25 known enzymes along the ERG production pathway. The effects of changes in expression of each ERG biosynthesis enzyme in Saccharomyces cerevisiae were analyzed by the use of gene deletion or plasmid-borne overexpression constructs. The strains overexpressing the ERG pathway genes were examined for changes in doubling time and responses to a variety of stress agents. In addition, ERG gene overexpression strains and ERG gene deletion strains were tested for alterations in antifungal drug susceptibility. The data show that disruptions in ergosterol biosynthesis regulation can affect a diverse set of cellular processes and can cause numerous phenotypic effects. Some of the phenotypes observed include dramatic increases in doubling times, respiratory deficiencies on glycerol media, cell wall insufficiencies on Congo red media, and disrupted ion homeostasis under iron or calcium starvation conditions. Overexpression or deletion of specific enzymes in the ERG pathway causes altered susceptibilities to a variety of classes of antifungal ergosterol inhibitors, including fluconazole, fenpropimorph, lovastatin, nystatin, amphotericin B, and terbinafine. This analysis of the effect of perturbations to the ERG pathway caused by systematic overexpression of each of the ERG pathway genes contributes significantly to the understanding of the ergosterol biosynthetic pathway and its relationship to stress response and basic biological processes. The data indicate that precise regulation of ERG genes is essential for cellular homeostasis and identify several ERG genes that could be exploited in future antifungal development efforts. IMPORTANCE A common target of antifungal drug treatment is the fungal ergosterol biosynthesis pathway. This report helps to identify ergosterol biosynthesis enzymes that have not previously been appreciated as drug targets. The effects of overexpression of each of the 25 ERG genes in S.?cerevisiae were analyzed in the presence of six stress agents that target essential cellular processes (cell wall biosynthesis, protein translation, respiration, osmotic/ionic stress, and iron and calcium homeostasis), as well as six antifungal inhibitors that target ergosterol biosynthesis. The importance of identifying cell perturbations caused by gene overexpression or deletion is emphasized by the prevalence of gene expression alterations in many pathogenic and drug-resistant clinical isolates. Genes whose altered expression causes the most extensive phenotypic alterations in the presence of stressors or inhibitors have the potential to be drug targets.
机译:摘要麦角固醇(ERG)是真菌细胞膜中的关键固醇,其生物合成受到沿ERG产生途径的25种已知酶的严格调控。通过使用基因缺失或质粒携带的过表达构建体,分析了酿酒酵母中每种ERG生物合成酶表达变化的影响。检查了过表达ERG途径基因的菌株的倍增时间变化以及对多种应激物质的反应。另外,测试了ERG基因过表达菌株和ERG基因缺失菌株的抗真菌药敏性。数据表明,麦角固醇生物合成调节的破坏会影响多种细胞过程,并可能导致许多表型效应。观察到的某些表型包括倍增时间的急剧增加,甘油培养基上的呼吸缺陷,刚果红培养基上的细胞壁不足以及在铁或钙饥饿条件下破坏了离子稳态。 ERG途径中特定酶的过度表达或缺失会导致对多种类型的抗真菌麦角固醇抑制剂(包括氟康唑,苯丙吗啡,洛伐他汀,制霉菌素,两性霉素B和特比萘芬)的敏感性改变。由每个ERG途径基因的系统性过表达引起的对ERG途径的扰动影响的分析,对理解麦角固醇生物合成途径及其与应激反应和基本生物学过程的关系有重要贡献。数据表明,ERG基因的精确调节对于细胞稳态是必不可少的,并确定了在未来的抗真菌开发工作中可以利用的几种ERG基因。重要事项抗真菌药物治疗的常见目标是真菌麦角固醇的生物合成途径。该报告有助于鉴定麦角固醇的生物合成酶,以前并未将其视为药物靶标。在六种针对基本细胞过程(细胞壁生物合成,蛋白质翻译,呼吸作用,渗透/离子应激以及铁和钙稳态)的应激剂的存在下,分析了酿酒酵母中25个ERG基因每个基因的过表达影响。 ),以及针对麦角固醇生物合成的六种抗真菌抑制剂。在许多致病性和耐药性临床分离株中,基因表达改变的普遍性强调了鉴定由基因过度表达或缺失引起的细胞扰动的重要性。在应激源或抑制剂存在下,表达改变的基因导致最广泛的表型改变,这些基因有可能成为药物靶标。

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