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冷诱导假定的DEAD盒RNA解旋酶CshA和CshB对枯草芽孢杆菌的冷适应至关重要,并与冷休克蛋白B相互作用。

Cold-induced putative DEAD box RNA helicases CshA and CshB are essential for cold adaptation and interact with cold shock protein B in Bacillus subtilis.

作者信息

Hunger Karen, Beckering Carsten L, Wiegeshoff Frank, Graumann Peter L, Marahiel Mohamed A

机构信息

Philipps-Universität Marburg, FB Chemie, Hans-Meerwein-Strasse, D-35032 Marburg, Germany.

出版信息

J Bacteriol. 2006 Jan;188(1):240-8. doi: 10.1128/JB.188.1.240-248.2006.

Abstract

The nucleic acid binding cold shock proteins (CSPs) and the cold-induced DEAD box RNA helicases have been proposed separately to act as RNA chaperones, but no experimental evidence has been reported on a direct cooperation. To investigate the possible interaction of the putative RNA helicases CshA and CshB and the CSPs from Bacillus subtilis during cold shock, we performed genetic as well as fluorescence resonance energy transfer (FRET) experiments. Both cshA and cshB genes could be deleted only in the presence of a cshB copy in trans, showing that the presence of one csh gene is essential for viability. The combined gene deletion of cshB and cspD resulted in a cold-sensitive phenotype that was not observed for either helicase or csp single mutants. In addition to the colocalization of the putative helicases CshA and CshB with CspB and the ribosomes in areas surrounding the nucleoid, we detected a strong FRET interaction in vivo between CshB and CspB that depended on active transcription. In contrast, a FRET interaction was not observed for CshB and the ribosomal protein L1. Therefore, we propose a model in which the putative cold-induced helicases and the CSPs work in conjunction to rescue misfolded mRNA molecules and maintain proper initiation of translation at low temperatures in B. subtilis.

摘要

核酸结合冷休克蛋白(CSPs)和冷诱导的DEAD盒RNA解旋酶曾被分别提出可作为RNA伴侣发挥作用,但尚未有关于它们直接协同作用的实验证据报道。为了研究枯草芽孢杆菌中假定的RNA解旋酶CshA和CshB与CSPs在冷休克期间可能的相互作用,我们进行了遗传学实验以及荧光共振能量转移(FRET)实验。只有在反式存在cshB拷贝的情况下,cshA和cshB基因才能被缺失,这表明一个csh基因的存在对于生存力至关重要。cshB和cspD的联合基因缺失导致了一种冷敏感表型,而单独的解旋酶或csp突变体均未观察到这种表型。除了假定的解旋酶CshA和CshB与CspB以及类核周围区域的核糖体共定位外,我们还在体内检测到CshB与CspB之间强烈的FRET相互作用,这种相互作用依赖于活跃转录。相比之下,未观察到CshB与核糖体蛋白L1之间的FRET相互作用。因此,我们提出了一个模型,即在枯草芽孢杆菌中,假定的冷诱导解旋酶和CSPs协同作用以挽救错误折叠的mRNA分子,并在低温下维持翻译的正确起始。

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