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A homologous overexpression system to study roles of drug transporters in Candida glabrata

机译:一种同源过度表达系统,用于研究念珠菌的药物转运蛋白的作用

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摘要

Considering the relevance of drug transporters belonging to ABC and MFS superfamilies in pathogenic Candida species, there has always been a need to have an overexpression system where these membrane proteins for functional analysis could be expressed in a homologous background. We could address this unmet need by constructing a highly drug-susceptible Candida glabrata strain deleted in seven dominant ABC transporters genes such as CgSNQ2, CgAUS1, CgCDR1, CgPDH1, CgYCF1, CgYBT1 and CgYOR1 and introduced a GOF mutation in transcription factor (TF) CgPDR1 leading to a hyper-activation of CgCDR1 locus. The expression system was validated by overexpressing four GFP tagged ABC (CgCDR1, CgPDH1, CaCDR1 and ScPDR5) and anMFS (CgFLR1) transporters genes facilitated by an engineered expression plasmid to integrate at the CgCDR1 locus. The properly expressed and localized transporters were fully functional, as was revealed by their several-fold increased drug resistance, growth kinetics, localization studies and efflux activities. The present homologous system will facilitate in determining the role of an individual transporter for its substrate specificity, drug efflux, pathogenicity and virulence traits without the interference of other major transporters.
机译:考虑到属于ABC和MFS Superfilies在病原念珠菌种类的药物转运蛋白的相关性,始终需要具有过表达系统,其中这些用于功能分析的膜蛋白可以在同源背景中表达。我们可以通过构建在七种显性ABC转运蛋白基因如CGSNQ2,CGAUS1,CGCDR1,CGPDH1,CGYCF1,CGG1和CGYOR1中删除的高毒易感念珠菌菌株来解决这种未满足的需求,并在转录因子(TF)CGPDR1中引入了GOF突变导致CGCDR1基因座的超激活。通过过表达四个GFP标记的ABC(CGCDR1,CGPDH1,CACDR1和SCPDR5)和通过工程表达质粒促进的ANMF(CGFLR1)转运蛋白基因来验证表达系统,以在CGCDR1基因座上整合。正确表达和局部的转运蛋白是完全函数的,正如其几倍增加的耐药,生长动力学,局部化研究和流出活动所揭示的那样。本同源系统将有助于确定单个转运蛋白的作用,用于其底物特异性,药物流出,致病性和毒力性状,而不会干扰其他主要运输术。

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