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大肠杆菌起始因子IF2β的串联翻译:两种活性形式的体外纯化与表征

Tandem translation of E. coli initiation factor IF2 beta: purification and characterization in vitro of two active forms.

作者信息

Nyengaard N R, Mortensen K K, Lassen S F, Hershey J W, Sperling-Petersen H U

机构信息

Dept. of Chemistry, Aarhus University, Denmark.

出版信息

Biochem Biophys Res Commun. 1991 Dec 31;181(3):1572-9. doi: 10.1016/0006-291x(91)92118-4.

Abstract

Two forms of E. coli initiation factor IF2, IF2 alpha and IF2 beta, have been known for several years. Both forms are products of the gene infB with translational initiation at codon 1 (AUG) and codon 158 (GUG) in the same reading frame. In this work we demonstrate that IF2 beta exists in two forms, IF2 beta and IF2 beta' with initiation codons 158 (GUG) and 165 (AUG) and molecular masses of 79.7 kDa and 78.8 kDa respectively. We have recently described a fast purification method for IF2 alpha, using an FPLC procedure consisting of ion-exchange liquid chromatography on Q Sepharose HP, Mono Q and Mono S. After the Mono Q step, an apparently homogeneous IF2 beta was observed when analyzed by SDS-PAGE. However the chromatography on Mono S results in the elution of two peaks containing IF2 beta. The N-terminal amino acid sequence of the two proteins identified the first peak to be IF2 beta and the second as a protein which we term IF2 beta' starting seven residues downstream at the AUG codon 165. The activity in vitro of the two purified forms of IF2 beta was tested by measuring the stimulation of binding of the initiator fMet-tRNA(fMet) to 70S ribosomes in the presence of GTP and poly(A,U,G) as messenger-RNA. In this assay no difference in activity is detected.

摘要

大肠杆菌起始因子IF2的两种形式,即IF2α和IF2β,已经为人所知数年。这两种形式都是infB基因的产物,在同一阅读框中分别从密码子1(AUG)和密码子158(GUG)开始翻译。在这项工作中,我们证明IF2β以两种形式存在,即IF2β和IF2β',起始密码子分别为158(GUG)和165(AUG),分子量分别为79.7 kDa和78.8 kDa。我们最近描述了一种IF2α的快速纯化方法,使用一种FPLC程序,该程序包括在Q Sepharose HP、Mono Q和Mono S上进行离子交换液相色谱。在Mono Q步骤之后,通过SDS-PAGE分析时观察到一种明显均一的IF2β。然而,在Mono S上的色谱分离导致洗脱含有IF2β的两个峰。这两种蛋白质的N端氨基酸序列确定第一个峰为IF2β,第二个峰为一种我们称为IF2β'的蛋白质,它在AUG密码子165处从下游七个残基处开始。通过在GTP和作为信使RNA的聚(A,U,G)存在下测量起始甲硫氨酰-tRNA(fMet)与70S核糖体结合的刺激作用,测试了两种纯化形式的IF2β的体外活性。在该测定中未检测到活性差异。

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