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核糖体亚基间桥B2a参与依赖因子的翻译起始和翻译持续性。

Ribosomal intersubunit bridge B2a is involved in factor-dependent translation initiation and translational processivity.

作者信息

Kipper Kalle, Hetényi Csaba, Sild Sulev, Remme Jaanus, Liiv Aivar

机构信息

Institute of Molecular and Cell Biology, University of Tartu, Riia 23, 51010 Tartu, Estonia.

出版信息

J Mol Biol. 2009 Jan 16;385(2):405-22. doi: 10.1016/j.jmb.2008.10.065. Epub 2008 Nov 5.

DOI:10.1016/j.jmb.2008.10.065
PMID:19007789
Abstract

Intersubunit bridges are important for holding together subunits in the 70S ribosome. Moreover, a number of intersubunit bridges have a role in modulating the activity of the ribosome during translation. Ribosomal intersubunit bridge B2a is formed by the interaction between the conserved 23S rRNA helix-loop 69 (H69) and the top of the 16S rRNA helix 44. Within the 70S ribosome, bridge B2a contacts translation factors and the A-site tRNA. In addition to bridging the subunits, bridge B2a has been invoked in a number of other ribosomal functions from initiation to termination. In the present work, single-nucleotide substitutions were inserted at positions 1912 and 1919 of Escherichia coli 23S rRNA (helix 69), which are involved in important intrahelical and intersubunit tertiary interactions in bridge B2a. The resulting ribosomes had a severely reduced activity in a cell-free translation elongation assay, but displayed a nearly wild-type-level peptidyl transferase activity. In vitro reassociation efficiency decreased with all of the H69 variant 50S subunits, but was severest with the A1919C and DeltaH69 variants. The mutations strongly affected initiation-factor-dependent 70S initiation complex formation, but exhibited a minor effect on the nonenzymatic initiation process. The mutations decreased ribosomal processivity in vitro and caused a progressive depletion of 50S subunits in polysomal fractions in vivo. Mutations at position 1919 decreased the stability of a dipeptidyl-tRNA in the A-site, whereas the binding of the dipeptidyl-tRNA was rendered more stable with 1912 and DeltaH69 mutations. Our results suggest that the H69 of 23S rRNA functions as a control element during enzymatic steps of translation.

摘要

亚基间桥对于70S核糖体中各亚基的结合非常重要。此外,一些亚基间桥在翻译过程中对核糖体活性的调节起作用。核糖体亚基间桥B2a由保守的23S rRNA螺旋-环69(H69)与16S rRNA螺旋44顶部之间的相互作用形成。在70S核糖体中,桥B2a与翻译因子和A位点tRNA接触。除了连接亚基外,桥B2a还参与了从起始到终止的许多其他核糖体功能。在本研究中,在大肠杆菌23S rRNA(螺旋69)的1912和1919位点插入了单核苷酸替换,这些位点参与桥B2a中重要的螺旋内和亚基间三级相互作用。在无细胞翻译延伸试验中,所得核糖体的活性严重降低,但显示出接近野生型水平的肽基转移酶活性。所有H69变体50S亚基的体外重新结合效率均降低,但A1919C和DeltaH69变体的降低最为严重。这些突变强烈影响起始因子依赖性70S起始复合物的形成,但对非酶促起始过程的影响较小。这些突变降低了体外核糖体的持续合成能力,并导致体内多核糖体组分中50S亚基的逐渐消耗。1919位点的突变降低了A位点二肽基-tRNA的稳定性,而1912和DeltaH69突变使二肽基-tRNA的结合更稳定。我们的结果表明,23S rRNA的H69在翻译的酶促步骤中起控制元件的作用。

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