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利用同步加速器产生的羟基自由基追踪核糖体亚基结合过程中16 S和23 S rRNA溶剂可及性的变化动态。

Following the dynamics of changes in solvent accessibility of 16 S and 23 S rRNA during ribosomal subunit association using synchrotron-generated hydroxyl radicals.

作者信息

Nguyenle Thuylinh, Laurberg Martin, Brenowitz Michael, Noller Harry F

机构信息

Center for Molecular Biology of RNA and Department of Molecular, Cell and Developmental Biology, University of California, Santa Cruz, 95064, USA.

出版信息

J Mol Biol. 2006 Jun 23;359(5):1235-48. doi: 10.1016/j.jmb.2006.04.030. Epub 2006 May 2.

Abstract

We have probed the structure and dynamics of ribosomal RNA in the Escherichia coli ribosome using equilibrium and time-resolved hydroxyl radical (OH) RNA footprinting to explore changes in the solvent-accessible surface of the rRNA with single-nucleotide resolution. The goal of these studies is to better understand the structural transitions that accompany association of the 30 S and 50 S subunits and to build a foundation for the quantitative analysis of ribosome structural dynamics during translation. Clear portraits of the subunit interface surfaces for 16 S and 23 S rRNA were obtained by constructing difference maps between the OH protection maps of the free subunits and that of the associated ribosome. In addition to inter-subunit contacts consistent with the crystal structure, additional OH protections are evident in regions at or near the subunit interface that reflect association-induced conformational changes. Comparison of these data with the comparable difference maps of the solvent-accessible surface of the rRNA calculated for the Thermus thermophilus X-ray crystal structures shows extensive agreement but also distinct differences. As a prelude to time-resolved OH footprinting studies, the reactivity profiles obtained using Fe(II)EDTA and X-ray generated OH were comprehensively compared. The reactivity patterns are similar except for a small number of nucleotides that have decreased reactivity to OH generated from Fe(II)EDTA compared to X-rays. These nucleotides are generally close to ribosomal proteins, which can quench diffusing radicals by virtue of side-chain oxidation. Synchrotron X-ray OH footprinting was used to monitor the kinetics of association of the 30 S and 50 S subunits. The rates individually measured for the inter-subunit contacts are comparable within experimental error. The application of this approach to the study of ribosome dynamics during the translation cycle is discussed.

摘要

我们利用平衡态和时间分辨羟基自由基(OH)RNA足迹法,探测了大肠杆菌核糖体中核糖体RNA的结构和动力学,以单核苷酸分辨率探索rRNA溶剂可及表面的变化。这些研究的目的是更好地理解30 S和50 S亚基缔合时伴随的结构转变,并为翻译过程中核糖体结构动力学的定量分析奠定基础。通过构建游离亚基和缔合核糖体的OH保护图谱之间的差异图谱,获得了16 S和23 S rRNA亚基界面表面的清晰图像。除了与晶体结构一致的亚基间接触外,在亚基界面处或其附近的区域还明显存在额外的OH保护,这反映了缔合诱导的构象变化。将这些数据与嗜热栖热菌X射线晶体结构计算得到的rRNA溶剂可及表面的可比差异图谱进行比较,结果显示出广泛的一致性,但也存在明显差异。作为时间分辨OH足迹研究的前奏,对使用Fe(II)EDTA和X射线产生的OH获得的反应性图谱进行了全面比较。除了少数核苷酸对Fe(II)EDTA产生的OH的反应性比X射线降低外,反应模式相似。这些核苷酸通常靠近核糖体蛋白,核糖体蛋白可通过侧链氧化淬灭扩散的自由基。同步加速器X射线OH足迹法用于监测30 S和50 S亚基的缔合动力学。在实验误差范围内,亚基间接触的单独测量速率具有可比性。本文还讨论了这种方法在翻译循环中核糖体动力学研究中的应用。

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