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核糖体蛋白转录途径的进化重布线改变了转录因子异二聚体 Ifh1-Fhl1(与 forkhead 1-forkhead-like 1 相互作用)与 DNA 结合特异性元件的相互作用。

The evolutionary rewiring of the ribosomal protein transcription pathway modifies the interaction of transcription factor heteromer Ifh1-Fhl1 (interacts with forkhead 1-forkhead-like 1) with the DNA-binding specificity element.

机构信息

Centre for Structural and Functional Genomics, Biology Department, Concordia University, Montréal, Québec H4B 1R6, Canada.

出版信息

J Biol Chem. 2013 Jun 14;288(24):17508-19. doi: 10.1074/jbc.M112.436683. Epub 2013 Apr 26.

DOI:10.1074/jbc.M112.436683
PMID:23625919
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3682550/
Abstract

The genes encoding the ribosomal proteins of fungi form a regulon whose expression is enhanced under good growth conditions and down-regulated under starvation conditions. The fungal pathogen Candida albicans contains an evolutionarily ancient control circuit for this regulon where a heteromer made up of the transcription regulators Ifh1 (interacts with Forkhead 1) and Fhl1 (Forkhead-like 1) is targeted to the ribosomal protein genes by the DNA binding factor Tbf1. In the more recently evolved circuit in the model yeast Saccharomyces cerevisiae (Sc), the generalist repressor-activator protein Rap1 now directs the Ifh1-Fhl1 module to the ribosomal protein genes. Even though overall sequence similarity is low for the respective Fhl1 and Ifh1 subunits, in both species, the Ifh1 protein links to the Forkhead-associated domain of Fhl1 through its FHB domain. Intriguingly, correlated with the transition to the Rap1-regulated circuit, the Sc-Ifh1 contains a Rap1 binding domain that is not present in the C. albicans protein. Because no extensive common sequences are found in Tbf1 and Rap1, it appears that these targeting proteins must connect to the Ifh1-Fhl1 module in distinct ways. Two-hybrid and co-immunoprecipitation analysis has been used to show that in C. albicans Tbf1 is linked to the heterodimer through direct association with Fhl1. By contrast, in S. cerevisiae, the linkage of the heteromer to Rap1 occurs through Ifh1. Thus, in the ascomycetes, the Ifh1-Fhl1 heterodimer has reconfigured its protein associations to remain connected to the ribosomal protein regulon despite rewiring of the targeting transcription factor from Tbf1 to Rap1.

摘要

真菌核糖体蛋白基因形成一个调控单元,其表达在良好的生长条件下增强,在饥饿条件下下调。真菌病原体白色念珠菌(Candida albicans)含有一个古老的控制回路,其中转录调节因子 Ifh1(与 Forkhead 1 相互作用)和 Fhl1(Forkhead-like 1)组成的异二聚体由 DNA 结合因子 Tbf1 靶向核糖体蛋白基因。在模式酵母酿酒酵母(Saccharomyces cerevisiae)中,进化上较新的回路中,通用抑制剂激活蛋白 Rap1 现在将 Ifh1-Fhl1 模块导向核糖体蛋白基因。尽管各自的 Fhl1 和 Ifh1 亚基的整体序列相似性较低,但在这两个物种中,Ifh1 蛋白通过其 FHB 结构域与 Fhl1 的 Forkhead 相关结构域连接。有趣的是,与向 Rap1 调节回路的转变相关,Sc-Ifh1 包含一个 Rap1 结合结构域,而该结构域不存在于 C. albicans 蛋白中。由于在 Tbf1 和 Rap1 中没有发现广泛的共同序列,因此这些靶向蛋白似乎必须以不同的方式连接到 Ifh1-Fhl1 模块。双杂交和共免疫沉淀分析已被用于表明在白色念珠菌中,Tbf1 通过与 Fhl1 的直接关联与异二聚体相连。相比之下,在酿酒酵母中,异二聚体与 Rap1 的连接通过 Ifh1 发生。因此,在子囊菌中,尽管靶向转录因子从 Tbf1 重布线到 Rap1,但 Ifh1-Fhl1 异二聚体已重新配置其蛋白质关联,以保持与核糖体蛋白调控单元的连接。

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