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通过Mcm1p结合位点对编码药物外排决定簇的MDR1进行转录调控,该调控存在于氟康唑耐药的白色念珠菌菌株中。

Transcriptional regulation of MDR1, encoding a drug efflux determinant, in fluconazole-resistant Candida albicans strains through an Mcm1p binding site.

作者信息

Riggle Perry J, Kumamoto Carol A

机构信息

Department of Molecular Biology and Microbiology, Tufts University School of Medicine, 136 Harrison Ave., Boston, MA 02111, USA.

出版信息

Eukaryot Cell. 2006 Dec;5(12):1957-68. doi: 10.1128/EC.00243-06. Epub 2006 Oct 13.

Abstract

Constitutive, high-level transcription of the gene encoding the drug efflux facilitator Mdr1p is commonly observed in laboratory and clinical strains of Candida albicans that are resistant to the antifungal drug fluconazole (FLC). In five independently isolated FLC(R) laboratory strains, introduction of a wild-type MDR1 promoter fragment fused to the yeast enhanced green fluorescent protein (yEGFP) reporter gene resulted in high-level expression of GFP, demonstrating that overexpression of MDR1 is dependent on a trans-acting factor. This study identified a 35-bp MDR1 promoter element, termed the MDRE, that mediates high-level MDR1 transcription. When inserted into a heterologous promoter, the MDRE was sufficient to mediate high-level expression of the yEGFP reporter gene specifically in MDR1 trans-activation strains. The MDRE promoted transcription in an orientation-independent and dosage-dependent manner. Deletion of the MDRE in the full-length promoter did not abolish MDR1 trans-activation, indicating that elements upstream of the MDRE also contribute to transcription of MDR1 in these overexpression strains. Analysis of the MDRE sequence indicated that it contains an Mcm1p binding site very similar in organization to the site seen upstream of the Saccharomyces cerevisiae MFA1 and STE2 genes. Electrophoretic mobility shift analysis demonstrated that both wild-type, FLC-sensitive and MDR1 trans-activated, FLC-resistant strains contain a factor that binds the MDRE. Depletion of Mcm1p, by use of a strain in which MCM1 expression is under the control of a regulated promoter (44), resulted in a loss of MDRE binding activity. Thus, the general transcription factor Mcm1p participates in the regulation of MDR1 expression.

摘要

在对抗真菌药物氟康唑(FLC)耐药的白色念珠菌实验室菌株和临床菌株中,通常可观察到编码药物外排促进因子Mdr1p的基因的组成型、高水平转录。在五个独立分离的FLC耐药实验室菌株中,将与酵母增强型绿色荧光蛋白(yEGFP)报告基因融合的野生型MDR1启动子片段导入后,导致GFP高水平表达,表明MDR1的过表达依赖于一种反式作用因子。本研究鉴定出一个35 bp的MDR1启动子元件,称为MDRE,它介导MDR1的高水平转录。当插入到异源启动子时,MDRE足以介导yEGFP报告基因在MDR1反式激活菌株中特异性高水平表达。MDRE以方向独立和剂量依赖的方式促进转录。全长启动子中MDRE的缺失并未消除MDR1的反式激活,表明MDRE上游的元件也有助于这些过表达菌株中MDR1的转录。对MDRE序列的分析表明,它包含一个与酿酒酵母MFA1和STE2基因上游位点组织非常相似的Mcm1p结合位点。电泳迁移率变动分析表明,野生型、FLC敏感型和MDR1反式激活的FLC耐药菌株均含有一种与MDRE结合的因子。通过使用一种MCM1表达受调控启动子控制的菌株(44)耗尽Mcm1p,导致MDRE结合活性丧失。因此,一般转录因子Mcm1p参与MDR1表达的调控。

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