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Adr1 介导了过氧化物酶体基因表达对 Snf1 的依赖性。

Snf1 dependence of peroxisomal gene expression is mediated by Adr1.

机构信息

Department of Biochemistry, University of Washington, Seattle, Washington 98195-7350, USA.

出版信息

J Biol Chem. 2010 Apr 2;285(14):10703-14. doi: 10.1074/jbc.M109.079848. Epub 2010 Feb 6.

Abstract

Eukaryotes utilize fatty acids by beta-oxidation, which occurs in the mitochondria and peroxisomes in higher organisms and in the peroxisomes in yeast. The AMP-activated protein kinase regulates this process in mammalian cells, and its homolog Snf1, together with the transcription factors Adr1, Oaf1, and Pip2, regulates peroxisome proliferation and beta-oxidation in yeast. A constitutive allele of Adr1 (Adr1(c)) lacking the glucose- and Snf1-regulated phosphorylation substrate Ser-230 was found to be Snf1-independent for regulation of peroxisomal genes. In addition, it could compensate for and even suppress the requirement for Oaf1 or Pip2 for gene induction. Peroxisomal genes were found to be regulated by oleate in the presence of glucose, as long as Adr1(c) was expressed, suggesting that the Oaf1/Pip2 heterodimer is Snf1-independent. Consistent with this observation, Oaf1 binding to promoters in the presence of oleate was not reduced in a snf1Delta strain. Exploring the mechanism by which Adr1(c) permits Snf1-independent peroxisomal gene induction, we found that strength of promoter binding did not correlate with transcription, suggesting that stable binding is not a prerequisite for enhanced transcription. Instead, enhanced transcriptional activation and suppression of Oaf1, Pip2, and Snf1 by Adr1(c) may be related to the ability of Adr1(c) to suppress the requirement for and enhance the recruitment of transcriptional coactivators in a promoter- and growth medium-dependent manner.

摘要

真核生物通过β-氧化作用利用脂肪酸,该过程发生在高等生物的线粒体和过氧化物酶体以及酵母的过氧化物酶体中。在哺乳动物细胞中,AMP 激活的蛋白激酶调节这个过程,其同源物 Snf1 与转录因子 Adr1、Oaf1 和 Pip2 一起调节酵母中过氧化物酶体的增殖和β-氧化。发现 Adr1 的组成型等位基因(Adr1(c))缺失葡萄糖和 Snf1 调节的磷酸化底物 Ser-230,对于过氧化物酶体基因的调节是 Snf1 非依赖性的。此外,它可以补偿甚至抑制 Oaf1 或 Pip2 对基因诱导的需求。发现过氧化物酶体基因在葡萄糖存在的情况下被油酸调节,只要表达 Adr1(c),这表明 Oaf1/Pip2 异二聚体是 Snf1 非依赖性的。与这一观察结果一致,在 snf1Delta 菌株中,Oaf1 与启动子结合的结合在存在油酸的情况下并没有减少。为了探索 Adr1(c) 允许 Snf1 非依赖性过氧化物酶体基因诱导的机制,我们发现启动子结合的强度与转录没有相关性,这表明稳定的结合不是增强转录的先决条件。相反,Adr1(c) 增强转录激活和抑制 Oaf1、Pip2 和 Snf1 可能与 Adr1(c) 以启动子和生长培养基依赖的方式抑制对转录共激活因子的需求并增强募集的能力有关。

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本文引用的文献

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Biochem Biophys Res Commun. 2008 Oct 3;374(4):763-6. doi: 10.1016/j.bbrc.2008.07.105. Epub 2008 Jul 29.
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