Kimball S R
Department of Cellular and Molecular Physiology, Pennsylvania State University College of Medicine, Hershey, Pennsylvania 17033, USA.
Prog Mol Subcell Biol. 2001;26:155-84. doi: 10.1007/978-3-642-56688-2_6.
The translation of mRNA in eukaryotic cells is regulated by amino acids through multiple mechanisms. One such mechanism involves activation of mTOR (Fig. 1). mTOR controls a myriad of downstream effectors, including RNA polymerase I, S6K1, 4E-BP1, and eEF2 kinase. In yeast, and probably in higher eukaryotes, mTOR signals through Tap42p/alpha 4 to regulate protein phosphatases. Through phosphorylation of Tap42p/alpha 4, mTOR abrogates dephosphorylation of the downstream effectors by PP2 A and/or PP6, resulting in their increased phosphorylation. Although at this time still speculative, in vitro results using mTOR immunoprecipitates suggest that mTOR, or an associated kinase, may also be directly involved in phosphorylating some effectors. Enhanced RNA polymerase I activity results in increased transcription of rDNA genes, whereas increased S6K1 activity promotes preferential translation of TOP mRNAs, such as those encoding ribosomal proteins. Together, stimulated RNA polymerase I and S6K1 activities enhance ribosome biogenesis, increasing the translational capacity of the cell. Phosphorylation of 4E-BP1 prohibits its association with eIF4E, allowing eIF4E to bind to eIF4G and form the active eIF4F complex. Increased eIF4F formation preferentially stimulates translation of mRNAs containing long, highly-structured 5' UTRs. Finally, amino acids cause inhibition of the eEF2 kinase, resulting in an increase in the proportion of eEF2 in the active, dephosphorylated form. By inhibiting eEF2 phosphorylation, amino acids may not only stimulate translation elongation, but may also prevent activation of GCN2 by enhancing the rate of removal of deacylated tRNA from the P-site on the ribosome; a potential activator of GCN2. GCN2 may also be regulated directly by the accumulation of deacylated-tRNA caused by treatment with inhibitors of tRNA synthetases or in cells incubated in the absence of essential amino acids. However, because the Km of the tRNA synthetases for amino acids is well above the amino acid concentrations found in plasma of fasted animals, such a mechanism may not be operative in mammals in vivo. Activation of GCN2 results in increased phosphorylation of the alpha-subunit of eIF2, which in turn causes inhibition of eIF2B. Thus, by preventing activation of GCN2, amino acids preserve eIF2B activity, which promotes translation of all mRNAs, i.e., global protein synthesis is enhanced.
真核细胞中mRNA的翻译受到氨基酸通过多种机制的调控。其中一种机制涉及mTOR的激活(图1)。mTOR控制着众多下游效应分子,包括RNA聚合酶I、S6K1、4E-BP1和eEF2激酶。在酵母中,可能在高等真核生物中也是如此,mTOR通过Tap42p/alpha 4发出信号来调节蛋白磷酸酶。通过对Tap42p/alpha 4的磷酸化,mTOR消除了PP2A和/或PP6对下游效应分子的去磷酸化作用,导致它们的磷酸化增加。尽管目前仍属推测,但使用mTOR免疫沉淀的体外实验结果表明,mTOR或相关激酶也可能直接参与某些效应分子的磷酸化。RNA聚合酶I活性增强导致rDNA基因转录增加,而S6K1活性增加则促进TOP mRNA(如编码核糖体蛋白的mRNA)的优先翻译。总之,受刺激的RNA聚合酶I和S6K1活性增强了核糖体生物合成,提高了细胞的翻译能力。4E-BP1的磷酸化阻止其与eIF4E结合,使eIF4E能够与eIF4G结合并形成活性eIF4F复合物。eIF4F形成增加优先刺激含有长的、高度结构化5'UTR的mRNA的翻译。最后,氨基酸导致eEF2激酶受到抑制,导致活性的、去磷酸化形式的eEF2比例增加。通过抑制eEF2磷酸化,氨基酸不仅可以刺激翻译延伸,还可能通过提高核糖体P位点上去酰化tRNA的去除速率来防止GCN2的激活;GCN2的潜在激活剂。GCN2也可能直接受到用tRNA合成酶抑制剂处理或在缺乏必需氨基酸的条件下培养的细胞中去酰化tRNA积累的调节。然而,由于tRNA合成酶对氨基酸的Km远高于禁食动物血浆中的氨基酸浓度,这种机制在哺乳动物体内可能不起作用。GCN2的激活导致eIF2的α亚基磷酸化增加,进而导致eIF2B受到抑制。因此,通过防止GCN2的激活,氨基酸保留了eIF2B活性,这促进了所有mRNA的翻译,即整体蛋白质合成得到增强。
