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O-GlcNAcylation/phosphorylation 循环在丝氨酸 10 位控制 δ-乳转铁蛋白的转录活性和稳定性。

O-GlcNAcylation/phosphorylation cycling at Ser10 controls both transcriptional activity and stability of delta-lactoferrin.

机构信息

Unité de Glycobiologie Structurale et Fonctionnelle, Unité Mixte de Recherche 8576 CNRS, Université des Sciences et Technologies de Lille, IFR 147, 59655 Villeneuve d'Ascq, France.

出版信息

J Biol Chem. 2010 Jun 18;285(25):19205-18. doi: 10.1074/jbc.M109.080572. Epub 2010 Apr 19.

Abstract

Delta-lactoferrin (DeltaLf) is a transcription factor that up-regulates DcpS, Skp1, and Bax genes, provoking cell cycle arrest and apoptosis. It is post-translationally modified either by O-GlcNAc or phosphate, but the effects of the O-GlcNAc/phosphorylation interplay on DeltaLf function are not yet understood. Here, using a series of glycosylation mutants, we showed that Ser(10) is O-GlcNAcylated and that this modification is associated with increased DeltaLf stability, achieved by blocking ubiquitin-dependent proteolysis, demonstrating that O-GlcNAcylation protects against polyubiquitination. We highlighted the (391)KSQQSSDPDPNCVD(404) sequence as a functional PEST motif responsible for DeltaLf degradation and defined Lys(379) as the main polyubiquitin acceptor site. We next investigated the control of DeltaLf transcriptional activity by the O-GlcNAc/phosphorylation interplay. Reporter gene analyses using the Skp1 promoter fragment containing a DeltaLf response element showed that O-GlcNAcylation at Ser(10) negatively regulates DeltaLf transcriptional activity, whereas phosphorylation activates it. Using a chromatin immunoprecipitation assay, we showed that O-GlcNAcylation inhibits DNA binding. Deglycosylation leads to DNA binding and transactivation of the Skp1 promoter at a basal level. Basal transactivation was markedly enhanced by 2-3-fold when phosphorylation was mimicked at Ser(10) by aspartate. Moreover, using double chromatin immunoprecipitation assays, we showed that the DeltaLf transcriptional complex binds to the DeltaLf response element and is phosphorylated and/or ubiquitinated, suggesting that DeltaLf transcriptional activity and degradation are concomitant events. Collectively, our results indicate that reciprocal occupancy of Ser(10) by either O-phosphate or O-GlcNAc coordinately regulates DeltaLf stability and transcriptional activity.

摘要

δ-乳白蛋白(DeltaLf)是一种转录因子,可上调 DcpS、Skp1 和 Bax 基因,引起细胞周期停滞和细胞凋亡。它可被 O-GlcNAc 或磷酸化进行翻译后修饰,但 O-GlcNAc/磷酸化相互作用对 DeltaLf 功能的影响尚不清楚。在这里,我们使用一系列糖基化突变体表明,丝氨酸(Ser)10 被 O-GlcNAc 化,这种修饰与 DeltaLf 稳定性的增加有关,这是通过阻止泛素依赖性蛋白水解来实现的,表明 O-GlcNAc 化可以防止多泛素化。我们强调了(391)KSQQSSDPDPNCVD(404)序列是一个功能性 PEST 基序,负责 DeltaLf 的降解,并确定了赖氨酸(Lys)379 是主要的多泛素接受位点。接下来,我们研究了 O-GlcNAc/磷酸化相互作用对 DeltaLf 转录活性的控制。使用含有 DeltaLf 反应元件的 Skp1 启动子片段进行报告基因分析表明,Ser(10)的 O-GlcNAc 化负调控 DeltaLf 转录活性,而磷酸化则激活它。使用染色质免疫沉淀测定,我们表明 O-GlcNAc 化抑制 DNA 结合。去糖基化导致 Skp1 启动子在基础水平上的 DNA 结合和反式激活。当 Ser(10)的磷酸化通过天冬氨酸模拟时,基础反式激活增强了 2-3 倍。此外,使用双染色质免疫沉淀测定,我们表明 DeltaLf 转录复合物与 DeltaLf 反应元件结合,并发生磷酸化和/或泛素化,表明 DeltaLf 转录活性和降解是伴随事件。总之,我们的结果表明,Ser(10)被 O-磷酸或 O-GlcNAc 共同占据,协调调节 DeltaLf 的稳定性和转录活性。

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