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血红素对喂食型和赖氨酸衍生型艾氏腹水肿瘤细胞无细胞提取物中蛋白质合成的翻译控制的影响。

The effects of haem on translational control of protein synthesis in cell-free extracts from fed and lysine-derived Ehrlich ascites tumour cells.

作者信息

Austin S A, Clemens M J

出版信息

Eur J Biochem. 1981 Jul;117(3):601-7. doi: 10.1111/j.1432-1033.1981.tb06380.x.

Abstract
  1. Addition of haem to cell-free extracts from Ehrlich ascites tumour cells stimulates protein synthesis only in extracts from cells previously incubated in nutritionally complete conditions. Extracts from amino-acid-deprived cells do not respond to haem. The stimulation of protein synthesis in fed cell extracts is due to increased initiation on endogenous mRNA mediated by an increase in the levels of 40-S-subunit X Met-tRNA initiation complexes. Extracts from starved cells exhibit a defect in 40-S initiation complex formation which cannot be overcome by haem. 2. Experiments to test for the presence of an inhibitor of initiation in Ehrlich cell extracts by monitoring effects on translation in haem-supplemented reticulocyte lysates have revealed that extracts from both fed and starved cells contain one or more inhibitory activities which shut off protein synthesis, dissagregate polysomes and reduce the level of 40-S initiation complexes in the lysate. Extracts from starved cells are more inhibitory for protein synthesis than those from fed cells. 3. Initiation factor eIF-2 is phosphorylated by an endogenous Ehrlich cell protein kinase in vitro, but this occurs to the same extent in extracts from fed and starved cells. 4. We propose a possible model for the role of eIF-2 in the control of protein synthesis by amino acid supply in Ehrlich cells.
摘要
  1. 向艾氏腹水瘤细胞的无细胞提取物中添加血红素,仅能刺激来自先前在营养完全条件下孵育的细胞提取物中的蛋白质合成。来自氨基酸缺乏细胞的提取物对血红素无反应。喂食细胞提取物中蛋白质合成的刺激是由于内源性mRNA起始增加,这是由40-S亚基X Met-tRNA起始复合物水平的增加介导的。饥饿细胞的提取物在40-S起始复合物形成方面存在缺陷,血红素无法克服这一缺陷。2. 通过监测对添加血红素的网织红细胞裂解物中翻译的影响来测试艾氏细胞提取物中是否存在起始抑制剂的实验表明,喂食和饥饿细胞的提取物都含有一种或多种抑制活性,这些活性会阻断蛋白质合成、分解多核糖体并降低裂解物中40-S起始复合物的水平。饥饿细胞的提取物对蛋白质合成的抑制作用比喂食细胞的提取物更强。3. 起始因子eIF-2在体外被艾氏细胞内源性蛋白激酶磷酸化,但在喂食和饥饿细胞的提取物中发生的程度相同。4. 我们提出了一个关于eIF-2在艾氏细胞中通过氨基酸供应控制蛋白质合成作用的可能模型。

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