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网织红细胞中膜功能与蛋白质合成之间的相互作用。一种从网织红细胞膜中提取的蛋白质合成延伸阶段抑制剂。

Interaction between membrane functions and protein synthesis in reticulocytes. An elongation-stage inhibitor of protein synthesis extracted from the reticulocyte membrane.

作者信息

Wreschner D H, Herzberg M

出版信息

Biochem J. 1979 May 15;180(2):379-87. doi: 10.1042/bj1800379.

Abstract

A component of the reticulocyte cell membrane was found to inhibit protein synthesis severely in a reticulocyte lysate system. An investigation into the mode of action of the membrane inhibitor revealed the following facts. (1) The binding of the tertiary initiation complex (methionyl-tRNAfMet-Initiation Factor 2-GTP) to the 40S ribosomal subunit was unaffected by the membrane inhibitor. (2) The membrane component did not interfere with the binding of the 40S initiation complex to the AUG initiation codon and subsequent attachment of the 60S ribosomal subunit. (3) Elongation of the peptide chain, as assayed by peptidyl-puromycin formation, was markedly affected by the membrane inhibitor. Surprisingly, the membrane component caused a considerable increase in peptidyl-puromycin formation. (4) Reticulocyte ribosomes that had been reisolated by high-speed centrifugation, after preincubation with the membrane component, were found to be highly defective when assayed in a cell-free protein-synthesizing system. These results indicated that an extract of the reticulocyte cell membrane inhibited protein synthesis by interacting with the ribosome and thus interfered with the correct functions of the elongation stage of protein synthesis. The implications of this conclusion are discussed in the light of data showing that a highly purified preparation of the membrane inhibitor also displayed an endonucleolytic activity highly specific for 28S RNA.

摘要

在网织红细胞裂解液系统中发现,网织红细胞细胞膜的一种成分会严重抑制蛋白质合成。对这种膜抑制剂作用方式的研究揭示了以下事实。(1)三级起始复合物(甲硫氨酰 - tRNAfMet - 起始因子2 - GTP)与40S核糖体亚基的结合不受膜抑制剂影响。(2)膜成分不干扰40S起始复合物与AUG起始密码子的结合以及随后60S核糖体亚基的附着。(3)通过肽基 - 嘌呤霉素形成来检测,肽链的延伸受到膜抑制剂的显著影响。令人惊讶的是,膜成分导致肽基 - 嘌呤霉素的形成大幅增加。(4)在与膜成分预孵育后,通过高速离心重新分离的网织红细胞核糖体,在无细胞蛋白质合成系统中检测时发现存在高度缺陷。这些结果表明,网织红细胞细胞膜提取物通过与核糖体相互作用抑制蛋白质合成,从而干扰了蛋白质合成延伸阶段的正确功能。根据显示膜抑制剂的高纯度制剂对28S RNA也具有高度特异性的核酸内切酶活性的数据,讨论了这一结论的意义。

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