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外文期刊>The biochemical journal
>Nitric oxide mediates NMDA-induced persistent inhibition of protein synthesis through dephosphorylation of eukaryotic initiation factor 4E-binding protein 1 and eukaryotic initiation factor 4G proteolysis
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Nitric oxide mediates NMDA-induced persistent inhibition of protein synthesis through dephosphorylation of eukaryotic initiation factor 4E-binding protein 1 and eukaryotic initiation factor 4G proteolysis
pCerebral ischaemia causes long-lasting protein synthesis inhibition that is believed to contribute to brain damage. Energy depletion promotes translation inhibition during ischaemia, and the phosphorylation of eIF (eukaryotic initiation factor) 2α is involved in the translation inhibition induced by early ischaemia/reperfusion. However, the molecular mechanisms underlying prolonged translation down-regulation remain elusive. NMDA (iN/i-methyl-D-aspartate) excitotoxicity is also involved in ischaemic damage, as exposure to NMDA impairs translation and promotes the synthesis of NO (nitric oxide), which can also inhibit translation. In the present study, we investigated whether NO was involved in NMDA-induced protein synthesis inhibition in neurons and studied the underlying molecular mechanisms. NMDA and the NO donor DEA/NO (diethylamine–nitric oxide sodium complex) both inhibited protein synthesis and this effect persisted after a 30 min exposure. Treatments with NMDA or NO promoted calpain-dependent eIF4G cleavage and 4E-BP1 (eIF4E-binding protein 1) dephosphorylation and also abolished the formation of eIF4E–eIF4G complexes; however, they did not induce eIF2α phosphorylation. Although NOS (NO synthase) inhibitors did not prevent protein synthesis inhibition during 30 min of NMDA exposure, they did abrogate the persistent inhibition of translation observed after NMDA removal. NOS inhibitors also prevented NMDA-induced eIF4G degradation, 4E-BP1 dephosphorylation, decreased eIF4E–eIF4G-binding and cell death. Although the calpain inhibitor calpeptin blocked NMDA-induced eIF4G degradation, it did not prevent 4E-BP1 dephosphorylation, which precludes eIF4E availability, and thus translation inhibition was maintained. The present study suggests that eIF4G integrity and hyperphosphorylated 4E-BP1 are needed to ensure appropriate translation in neurons. In conclusion, our data show that NO mediates NMDA-induced persistent translation inhibition and suggest that deficient eIF4F activity contributes to this process./p
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机译:>脑缺血导致长期的蛋白质合成抑制作用,据信这会导致脑损伤。能量消耗促进局部缺血期间的翻译抑制,而eIF(真核起始因子)2α的磷酸化与早期局部缺血/再灌注诱导的翻译抑制有关。但是,延长翻译下调的潜在分子机制仍然难以捉摸。 NMDA( N -甲基-D-天冬氨酸)兴奋性毒性也与缺血性损伤有关,因为暴露于NMDA会损害翻译并促进NO(一氧化氮)的合成,而NO也可能抑制翻译。在本研究中,我们调查了NO是否参与NMDA诱导的神经元蛋白合成抑制,并研究了潜在的分子机制。 NMDA和NO供体DEA / NO(二乙胺-一氧化氮钠络合物)均抑制蛋白质合成,并且这种作用在暴露30分钟后仍然存在。 NMDA或NO的治疗促进了钙蛋白酶依赖性eIF4G裂解和4E-BP1(eIF4E结合蛋白1)的去磷酸化作用,也消除了eIF4E-eIF4G复合物的形成。但是,它们没有诱导eIF2α磷酸化。尽管NOS(NO合酶)抑制剂在NMDA暴露30分钟内并未阻止蛋白质合成抑制,但它们确实消除了NMDA去除后观察到的翻译的持续抑制。 NOS抑制剂还可以防止NMDA诱导的eIF4G降解,4E-BP1去磷酸化,eIF4E–eIF4G结合减少和细胞死亡。尽管钙蛋白酶抑制剂钙蛋白酶抑制了NMDA诱导的eIF4G降解,但是它并不能阻止4E-BP1的去磷酸化,从而阻止了eIF4E的可用性,因此可以维持翻译抑制作用。本研究表明,需要eIF4G完整性和磷酸化4E-BP1以确保神经元中的适当翻译。总之,我们的数据表明,NO不能介导NMDA诱导的持续翻译抑制,并表明eIF4F活性不足是这一过程的原因。
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