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通过实验与计算相结合的方法完善关于酵母FLR1调控网络的现有知识。

Refining current knowledge on the yeast FLR1 regulatory network by combined experimental and computational approaches.

作者信息

Teixeira M C, Dias P J, Monteiro P T, Sala A, Oliveira A L, Freitas A T, Sá-Correia I

机构信息

IBB-Institute for Biotechnology and BioEngineering, Centro de Engenharia Biológica e Química, Instituto Superior Técnico, Technical University of Lisbon, Av. Rovisco Pais, 1049-001 Lisboa, Portugal.

出版信息

Mol Biosyst. 2010 Dec;6(12):2471-81. doi: 10.1039/c004881j. Epub 2010 Oct 11.

Abstract

Multidrug resistance is often the result of the activation of drug efflux pumps able to catalyze the extrusion of the toxic compound to the outer medium, this activation being frequently controlled at the transcriptional level. Transcriptional regulation in the model eukaryote S. cerevisiae is the result of the interaction and cross-talk between networks of transcription factors. This is the case of the transcriptional activation of the FLR1 gene occurring in response to stress induced by the agricultural fungicide mancozeb in yeast. FLR1 up-regulation depends on the integrated action of Yap1, a key regulator of oxidative stress response, Pdr3 and Yrr1, two of the transcription factors controlling multidrug resistance, and Rpn4, a regulator of proteasome gene expression, which interplay to produce the observed transcriptional up-shift. Based on the expression profiles of FLR1, YAP1, PDR3, YRR1 and RPN4 registered during yeast adaptation to stress induced by mancozeb and using a qualitative modeling approach, a model of the FLR1 regulatory network was built, and the response of S. cerevisiae to mancozeb stress was simulated. The use of a qualitative approach is especially useful to overcome the lack of enough quantitative data on kinetic parameters and molecular concentrations, permitting the immediate focus on the qualitative behavior of the system. This Systems Biology approach allowed the identification of essential features of the early yeast response to fungicide stress. The resulting model allowed the formulation of new hypotheses, in a quick and cost effective manner, on the qualitative behavior of the system following mancozeb challenge, some of which were validated experimentally. In particular, Pdr3 and Yrr1 were shown to directly control FLR1 up-regulation in mancozeb-challenged cells, based on the analysis of the effect of the inactivation of their putative binding sites in the FLR1 promoter. Furthermore, the inter-dependent role of Yap1 and Yrr1 in the regulation of PDR3 and RPN4 was brought to light, this joint activity possibly being extensible to eight other genes involved in multidrug resistance. The FLR1 network structure was revised, based on the comparison between simulated and experimental gene expression data in the double deletion mutant strains Δyrr1Δpdr3 and Δyrr1Δrpn4, and an additional, still unidentified, transcription factor was found to be required to fully explain the behavior of the network.

摘要

多药耐药性通常是药物外排泵激活的结果,这些泵能够催化将有毒化合物排到细胞外环境中,这种激活常常在转录水平受到调控。在模式真核生物酿酒酵母中,转录调控是转录因子网络之间相互作用和相互影响的结果。农业杀菌剂代森锰锌在酵母中诱导产生应激反应时,FLR1基因的转录激活就是这种情况。FLR1的上调依赖于Yap1(氧化应激反应的关键调节因子)、Pdr3和Yrr1(控制多药耐药性的两个转录因子)以及Rpn4(蛋白酶体基因表达的调节因子)的综合作用,它们相互作用导致观察到的转录上调。基于酿酒酵母适应代森锰锌诱导的应激过程中记录的FLR1、YAP1、PDR3、YRR1和RPN4的表达谱,并采用定性建模方法,构建了FLR1调控网络模型,并模拟了酿酒酵母对代森锰锌应激的反应。使用定性方法对于克服动力学参数和分子浓度方面定量数据不足的问题特别有用,能够直接关注系统的定性行为。这种系统生物学方法有助于识别酵母对杀菌剂应激早期反应的基本特征。所得模型能够以快速且经济高效的方式就代森锰锌攻击后系统的定性行为提出新的假设,其中一些已通过实验验证。特别是,基于对FLR1启动子中其假定结合位点失活效应的分析,发现Pdr3和Yrr1可直接控制代森锰锌攻击细胞中FLR1的上调。此外,还揭示了Yap1和Yrr1在PDR3和RPN4调控中的相互依赖作用,这种联合活性可能扩展到其他八个参与多药耐药性的基因。基于双缺失突变菌株Δyrr1Δpdr3和Δyrr1Δrpn4中模拟和实验基因表达数据的比较,对FLR1网络结构进行了修订,发现还需要一个尚未鉴定的额外转录因子才能完全解释该网络的行为。

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