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使用[14C]真核起始因子2来测量兔网织红细胞裂解物中真核起始因子2的内源性库大小。

The use of [14C]eukaryotic initiation factor 2 to measure the endogenous pool size of eukaryotic initiation factor 2 in rabbit reticulocyte lysate.

作者信息

Safer B, Kemper W, Jagus R

出版信息

J Biol Chem. 1979 Sep 10;254(17):8091-4.

PMID:256941
Abstract

[14C]Eukaryotic initiation factor 2 (eIF-2), obtained by reductive methylation of the purified initiation factor, was shown to be active in the unfractionated reticulocyte lysate. This allowed a direct measurement of the endogenous pool size of eIF-2 in rabbit reticulocyte lysate according to the principle of isotope dilution. A value of 20 to 30 pmol/ml of lysate was obtained. Although translational inhibition resulting from hemin deficiency appears to be characterized by a change from catalytic to stoichiometric utilization of eIF-2, the pool size of eIF-2 is too small to account for the normal period of protein synthesis before the onset of translation inhibition. This suggests, therefore, that additional events to eIF-2 alpha phosphorylation may be required for translational inhibition.

摘要

通过对纯化的起始因子进行还原甲基化获得的[14C]真核起始因子2(eIF-2),在未分级的网织红细胞裂解物中显示出活性。这使得能够根据同位素稀释原理直接测量兔网织红细胞裂解物中eIF-2的内源性库大小。获得的裂解物值为20至30 pmol/ml。尽管血红素缺乏导致的翻译抑制似乎以eIF-2从催化利用转变为化学计量利用为特征,但eIF-2的库大小太小,无法解释翻译抑制开始前蛋白质合成的正常时期。因此,这表明翻译抑制可能需要eIF-2α磷酸化以外的其他事件。

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