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兔网织红细胞中的蛋白质合成。对Co-eIF-2作用机制的研究。

Protein synthesis in rabbit reticulocytes. A study of the mechanism of Co-eIF-2 action.

作者信息

Bagchi M K, Chakravarty I, Datta B, Chakrabarti D, Gupta N K

出版信息

J Biol Chem. 1985 Dec 5;260(28):14976-81.

PMID:3851808
Abstract

The characteristics of component activities in Co-eIF-2 (where eIF is eukaryotic initiation factor) protein complex have been studied. (i) At limiting concentrations, Co-eIF-2 promoted rapid GDP binding to eIF-2 and also GDP displacement from eIF-2 X GDP during ternary complex formation in the presence of GTP and Mg2+ (Co-eIF-2C activity) but did not significantly stimulate ternary complex formation by eIF-2. (ii) At higher concentrations, Co-eIF-2 significantly enhanced ternary complex formation by eIF-2 and also rendered the complex stable to aurintricarboxylic acid presumably as Co-eIF-2 became physically bound to the ternary complex (Co-eIF-2A activity). (iii) Ternary complex preformed in the presence of Co-eIF-2 and without Mg2+ dissociated upon subsequent addition of Mg2+ (Co-eIF-2B activity). This dissociation reaction was presumably due to loss of interaction of the Co-eIF-2A component in Co-eIF-2 with the ternary complex (reversal of Co-eIF-2A activity) as the complex became increasingly sensitive to aurintricarboxylic acid with increasing Mg2+ concentration. In another study, purified eIF-2 was freed of bound GDP by treatment with alkaline phosphatase and the characteristics of native and GDP-free eIF-2 were compared. (i) One mM Mg2+ inhibited (60%) ternary complex formation by native eIF-2 but not by GDP-free eIF-2. Addition of exogenous GDP rendered GDP-free eIF-2 sensitive to Mg2+ indicating that Mg2+ inhibition is due to eIF-2-bound GDP. (ii) In the presence of Mg2+, Co-eIF-2 stimulated similarly ternary and Met-tRNAf X 40 S X AUG complex formation by both native and GDP-free eIF-2. Such stimulatory activity in each case was strongly inhibited by prior phosphorylation of eIF-2 alpha subunit by heme-regulated translational inhibitor. (iii) Ternary complexes preformed using either native and GDP-free eIF-2 and excess Co-eIF-2A80 in the absence of Mg2+ did not form Met-tRNAf X 40 S X AUG complex. They required trace amounts of Co-eIF-2 for such activity.

摘要

对Co-eIF-2(其中eIF为真核起始因子)蛋白复合物中各组成活性的特征进行了研究。(i) 在极限浓度下,Co-eIF-2促进GDP与eIF-2快速结合,并且在存在GTP和Mg2+的三元复合物形成过程中,也促进GDP从eIF-2·GDP上置换下来(Co-eIF-2C活性),但并未显著刺激eIF-2形成三元复合物。(ii) 在较高浓度下,Co-eIF-2显著增强eIF-2形成三元复合物的能力,并且使该复合物对金精三羧酸稳定,推测这是由于Co-eIF-2与三元复合物发生了物理结合(Co-eIF-2A活性)。(iii) 在存在Co-eIF-2且无Mg2+的情况下预先形成的三元复合物,在随后加入Mg2+时会解离(Co-eIF-2B活性)。这种解离反应可能是由于随着Mg2+浓度增加,复合物对金精三羧酸越来越敏感,Co-eIF-2中的Co-eIF-2A组分与三元复合物的相互作用丧失(Co-eIF-2A活性的逆转)。在另一项研究中,用碱性磷酸酶处理纯化的eIF-2以去除结合的GDP,并比较了天然eIF-2和无GDP的eIF-2的特征。(i) 1 mM Mg2+抑制天然eIF-2形成三元复合物(60%),但不抑制无GDP的eIF-2。加入外源GDP使无GDP的eIF-2对Mg2+敏感,表明Mg2+的抑制作用是由于eIF-2结合的GDP。(ii) 在存在Mg2+的情况下,Co-eIF-2对天然eIF-2和无GDP的eIF-2形成三元复合物以及Met-tRNAf·40S·AUG复合物的刺激作用相似。在每种情况下,这种刺激活性都被血红素调节的翻译抑制剂对eIF-2α亚基的预先磷酸化强烈抑制。(iii) 使用在不存在Mg2+的情况下,使用天然eIF-2和无GDP的eIF-2以及过量Co-eIF-2A80预先形成的三元复合物不会形成Met-tRNAf·40S·AUG复合物。它们需要微量的Co-eIF-2才能有这种活性。

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