Department of Investigation, Hospital Ramón y Cajal, 28034 Madrid, Spain.
J Biol Chem. 2010 Nov 5;285(45):34355-63. doi: 10.1074/jbc.M110.135103. Epub 2010 Aug 24.
Eukaryotic initiation factor (eIF) 4E-binding protein 1 (4E-BP1) is a translational repressor that is characterized by its capacity to bind specifically to eIF4E and inhibit its interaction with eIF4G. Phosphorylation of 4E-BP1 regulates eIF4E availability, and therefore, cap-dependent translation, in cell stress. This study reports a physiological study of 4E-BP1 regulation by phosphorylation using control conditions and a stress-induced translational repression condition, ischemia-reperfusion (IR) stress, in brain tissue. In control conditions, 4E-BP1 was found in four phosphorylation states that were detected by two-dimensional gel electrophoresis and Western blotting, which corresponded to Thr(69)-phosphorylated alone, Thr(69)- and Thr(36)/Thr(45)-phosphorylated, all these plus Ser(64) phosphorylation, and dephosphorylation of the sites analyzed. In control or IR conditions, no Thr(36)/Thr(45) phosphorylation alone was detected without Thr(69) phosphorylation, and neither was Ser(64) phosphorylation without Thr(36)/Thr(45)/Thr(69) phosphorylation detected. Ischemic stress induced 4E-BP1 dephosphorylation at Thr(69), Thr(36)/Thr(45), and Ser(64) residues, with 4E-BP1 remaining phosphorylated at Thr(69) alone or dephosphorylated. In the subsequent reperfusion, 4E-BP1 phosphorylation was induced at Thr(36)/Thr(45) and Ser(64), in addition to Thr(69). Changes in 4E-BP1 phosphorylation after IR were according to those found for Akt and mammalian target of rapamycin (mTOR) kinases. These results demonstrate a new hierarchical phosphorylation for 4E-BP1 regulation in which Thr(69) is phosphorylated first followed by Thr(36)/Thr(45) phosphorylation, and Ser(64) is phosphorylated last. Thr(69) phosphorylation alone allows binding to eIF4E, and subsequent Thr(36)/Thr(45) phosphorylation was sufficient to dissociate 4E-BP1 from eIF4E, which led to eIF4E-4G interaction. These data help to elucidate the physiological role of 4E-BP1 phosphorylation in controlling protein synthesis.
真核起始因子 4E 结合蛋白 1(4E-BP1)是一种翻译抑制剂,其特征是能够特异性结合 eIF4E 并抑制其与 eIF4G 的相互作用。4E-BP1 的磷酸化调节细胞应激时 eIF4E 的可用性和因此帽依赖性翻译。本研究使用对照条件和应激诱导的翻译抑制条件(缺血再灌注(IR)应激)报告了 4E-BP1 磷酸化调节的生理研究,在脑组织中。在对照条件下,通过二维凝胶电泳和 Western blot 检测到 4E-BP1 的四种磷酸化状态,分别对应于 Thr(69)单独磷酸化、Thr(69)和 Thr(36)/Thr(45)磷酸化、所有这些加上 Ser(64)磷酸化以及分析的位点去磷酸化。在对照或 IR 条件下,未检测到 Thr(36)/Thr(45)磷酸化而不 Thr(69)磷酸化,也未检测到 Ser(64)磷酸化而不 Thr(36)/Thr(45)/Thr(69)磷酸化。缺血应激诱导 4E-BP1 在 Thr(69)、Thr(36)/Thr(45)和 Ser(64)残基上脱磷酸化,4E-BP1 仍在 Thr(69)上磷酸化或脱磷酸化。再灌注后,除 Thr(69)外,4E-BP1 在 Thr(36)/Thr(45)和 Ser(64)上被诱导磷酸化。IR 后 4E-BP1 磷酸化的变化与 Akt 和哺乳动物雷帕霉素靶蛋白(mTOR)激酶的变化一致。这些结果表明,4E-BP1 调节的新层次磷酸化,其中 Thr(69)首先磷酸化,然后 Thr(36)/Thr(45)磷酸化,最后 Ser(64)磷酸化。单独的 Thr(69)磷酸化允许与 eIF4E 结合,随后 Thr(36)/Thr(45)磷酸化足以使 4E-BP1 从 eIF4E 上解离,从而导致 eIF4E-4G 相互作用。这些数据有助于阐明 4E-BP1 磷酸化在控制蛋白质合成中的生理作用。
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