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GCN4的翻译调控因子GCN1和GCN20在激活eIF2α激酶GCN2的过程中作用于延伸中的核糖体的证据。

Evidence that GCN1 and GCN20, translational regulators of GCN4, function on elongating ribosomes in activation of eIF2alpha kinase GCN2.

作者信息

Marton M J, Vazquez de Aldana C R, Qiu H, Chakraburtty K, Hinnebusch A G

机构信息

Laboratory of Eukaryotic Gene Regulation, National Institute of Child Health and Human Development, Bethesda, Maryland 20892, USA.

出版信息

Mol Cell Biol. 1997 Aug;17(8):4474-89. doi: 10.1128/MCB.17.8.4474.

Abstract

In the yeast Saccharomyces cerevisiae, phosphorylation of translation initiation factor eIF2 by protein kinase GCN2 leads to increased translation of the transcriptional activator GCN4 in amino acid-starved cells. The GCN1 and GCN20 proteins are components of a protein complex required for the stimulation of GCN2 kinase activity under starvation conditions. GCN20 is a member of the ATP-binding cassette (ABC) family, most of the members of which function as membrane-bound transporters, raising the possibility that the GCN1/GCN20 complex regulates GCN2 indirectly as an amino acid transporter. At odds with this idea, indirect immunofluorescence revealed cytoplasmic localization of GCN1 and no obvious association with plasma or vacuolar membranes. In addition, a fraction of GCN1 and GCN20 cosedimented with polysomes and 80S ribosomes, and the ribosome association of GCN20 was largely dependent on GCN1. The C-terminal 84% of GCN20 containing the ABCs was found to be dispensable for complex formation with GCN1 and for the stimulation of GCN2 kinase function. Because ABCs provide the energy-coupling mechanism for ABC transporters, these results also contradict the idea that GCN20 regulates GCN2 as an amino acid transporter. The N-terminal 15 to 25% of GCN20, which is critically required for its regulatory function, was found to interact with an internal segment of GCN1 similar in sequence to translation elongation factor 3 (EF3). Based on these findings, we propose that GCN1 performs an EF3-related function in facilitating the activation of GCN2 by uncharged tRNA on translating ribosomes. The physical interaction between GCN20 and the EF3-like domain in GCN1 could allow for modulation of GCN1 activity, and the ABC domains in GCN20 may be involved in this regulatory function. A human homolog of GCN1 has been identified, and the portion of this protein most highly conserved with yeast GCN1 has sequence similarity to EF3. Thus, similar mechanisms for the detection of uncharged tRNA on translating ribosomes may operate in yeast and human cells.

摘要

在酿酒酵母中,蛋白激酶GCN2对翻译起始因子eIF2的磷酸化作用导致在氨基酸饥饿的细胞中转录激活因子GCN4的翻译增加。GCN1和GCN20蛋白是在饥饿条件下刺激GCN2激酶活性所需的蛋白复合物的组成成分。GCN20是ATP结合盒(ABC)家族的成员,该家族的大多数成员作为膜结合转运蛋白发挥作用,这增加了GCN1/GCN20复合物作为氨基酸转运蛋白间接调节GCN2的可能性。与这一观点相悖的是,间接免疫荧光显示GCN1定位于细胞质,与质膜或液泡膜无明显关联。此外,一部分GCN1和GCN20与多核糖体和80S核糖体共沉降,并且GCN20与核糖体的结合很大程度上依赖于GCN1。发现GCN20含有ABC结构域的C末端84%对于与GCN1形成复合物以及刺激GCN2激酶功能是可有可无的。由于ABC结构域为ABC转运蛋白提供能量偶联机制,这些结果也与GCN20作为氨基酸转运蛋白调节GCN2的观点相矛盾。发现GCN20的N末端15%至25%对其调节功能至关重要,它与GCN1的一个内部片段相互作用,该片段在序列上与翻译延伸因子3(EF3)相似。基于这些发现,我们提出GCN1在促进GCN2被翻译核糖体上的空载tRNA激活方面发挥与EF3相关的功能。GCN20与GCN1中EF3样结构域之间的物理相互作用可能允许调节GCN1的活性,并且GCN20中的ABC结构域可能参与这一调节功能。已鉴定出GCN1的人类同源物,该蛋白与酵母GCN1保守性最高的部分与EF3具有序列相似性。因此,在酵母和人类细胞中可能存在检测翻译核糖体上空载tRNA的类似机制。

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