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大肠杆菌Hfq的C末端结构域可提高六聚体的稳定性。

The C-terminal domain of Escherichia coli Hfq increases the stability of the hexamer.

作者信息

Arluison Véronique, Folichon Marc, Marco Sergio, Derreumaux Philippe, Pellegrini Olivier, Seguin Jérôme, Hajnsdorf Eliane, Regnier Philippe

机构信息

Institut de Biologie Physico-Chimique CNRS UPR 9073 conventionnée avec l'université Paris 7, Paris, France.

出版信息

Eur J Biochem. 2004 Apr;271(7):1258-65. doi: 10.1111/j.1432-1033.2004.04026.x.

DOI:10.1111/j.1432-1033.2004.04026.x
PMID:15030475
Abstract

The Hfq (Host factor 1) polypeptide is a nucleic acid binding protein involved in the synthesis of many polypeptides. Hfq particularly affects the translation and the stability of several RNAs. In an earlier study, the use of fold recognition methods allowed us to detect a relationship between Escherichia coli Hfq and the Sm topology. This topology was further validated by a series of biophysical studies and the Hfq structure was modelled on an Sm protein. Hfq forms a beta-sheet ring-shaped hexamer. As our previous study predicted a large number of alternative conformations for the C-terminal region, we have determined whether the last 19 C-terminal residues are necessary for protein function. We find that the C-terminal truncated protein is fully capable of binding a polyadenylated RNA (K(d) of 120 pm vs. 50 pm for full-length Hfq). This result shows that the functional core of E. coli Hfq resides in residues 1-70 and confirms previous genetic studies. Using equilibrium unfolding studies, however, we find that full-length Hfq is 1.8 kcal x mol(-1) more stable than its truncated variant. Electron microscopy analysis of both truncated and full-length proteins indicates a structural rearrangement between the subunits upon truncation. This conformational change is coupled to a reduction in beta-strand content, as determined by Fourier transform infra-red. On the basis of these results, we propose that the C-terminal domain could protect the interface between the subunits and stabilize the hexameric Hfq structure. The origin of this C-terminal domain is also discussed.

摘要

Hfq(宿主因子1)多肽是一种参与多种多肽合成的核酸结合蛋白。Hfq特别影响几种RNA的翻译和稳定性。在早期的一项研究中,使用折叠识别方法使我们能够检测到大肠杆菌Hfq与Sm拓扑结构之间的关系。通过一系列生物物理研究进一步验证了这种拓扑结构,并基于Sm蛋白对Hfq结构进行了建模。Hfq形成一个β-折叠环形六聚体。由于我们之前的研究预测了C末端区域的大量替代构象,我们确定了C末端的最后19个残基对于蛋白质功能是否必要。我们发现C末端截短的蛋白质完全能够结合多聚腺苷酸化RNA(全长Hfq的K(d)为50 pm,截短蛋白的K(d)为120 pm)。这一结果表明大肠杆菌Hfq的功能核心位于第1-70位残基,证实了之前的遗传学研究。然而,通过平衡去折叠研究,我们发现全长Hfq比其截短变体稳定1.8 kcal·mol⁻¹。对截短蛋白和全长蛋白的电子显微镜分析表明,截短后亚基之间发生了结构重排。如通过傅里叶变换红外光谱所确定的,这种构象变化与β-链含量的减少相关。基于这些结果,我们提出C末端结构域可以保护亚基之间的界面并稳定六聚体Hfq结构。我们还讨论了这个C末端结构域的起源。

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