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来自极端嗜盐古细菌红皮盐杆菌的两种延伸因子。高盐浓度下的测定系统与纯化。

Two elongation factors from the extremely halophilic archaebacterium Halobacterium cutirubrum. Assay systems and purification at high salt concentrations.

作者信息

Kessel M, Klink F

出版信息

Eur J Biochem. 1981 Mar;114(3):481-6. doi: 10.1111/j.1432-1033.1981.tb05170.x.

Abstract

Two peptide chain elongation factors from Halobacterium cutirubrum were purified nearly to homogeneity. They were identified and characterized by three assay systems working at very high salt concentrations: poly(Phe) synthesis, GDP binding and ADP-ribosylation. The purification procedure consisted of Sepharose 4B chromatography with a decreasing ammonium sulfate gradient, gel filtration on Sephadex G-100 in the presence of (NH4)2SO4 and, for each of the two separated factors, an independent adsorption chromatography on hydroxyapatite. The factors were absolutely dependent on high salt concentrations for stability and activity. Both factors (I and II) complement each other to give fully active poly(Phe) synthesis, which is totally inhibited by puromycin and anisomycin. Factor I (Mr 51 000) is a major protein of the cell-free extract. It binds GDP, which can be displaced by GTP only to a small extent. The function of factor I in poly(Phe) synthesis is not impaired by high concentrations of kirromycin. The observed characteristics resemble partly those of prokaryotic EF-Tu and partly those of eukaryotic EF-1. Factor II (Mr 111 000) can be ADP-ribosylated by diphtheria toxin, and thus was identified as an EF-2-type elongation factor.

摘要

从深红嗜盐菌中纯化出了两种肽链延长因子,纯度几乎达到均一。通过在非常高的盐浓度下工作的三种测定系统对它们进行了鉴定和表征:聚(苯丙氨酸)合成、GDP结合和ADP-核糖基化。纯化过程包括用递减的硫酸铵梯度进行琼脂糖4B层析、在硫酸铵存在下在葡聚糖G-100上进行凝胶过滤,以及对两个分离的因子分别进行独立的羟基磷灰石吸附层析。这些因子的稳定性和活性绝对依赖于高盐浓度。两个因子(I和II)相互补充,以实现完全活性的聚(苯丙氨酸)合成,而嘌呤霉素和茴香霉素可完全抑制该合成。因子I(Mr 51 000)是无细胞提取物中的主要蛋白质。它结合GDP,GTP只能少量取代GDP。高浓度的奇霉素不会损害因子I在聚(苯丙氨酸)合成中的功能。观察到的特征部分类似于原核生物的EF-Tu,部分类似于真核生物的EF-1。因子II(Mr 111 000)可被白喉毒素ADP-核糖基化,因此被鉴定为EF-2型延长因子。

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