Exploring ribozyme conformational changes with X-ray crystallography

被引:12
|
作者
Spitale, Robert C. [2 ]
Wedekind, Joseph E. [1 ,2 ]
机构
[1] Dept Biochem & Biophys, Rochester, NY 14642 USA
[2] Univ Rochester, Dept Chem, Biol Chem Cluster, Rochester, NY 14627 USA
关键词
RNA crystallography; Ribozyme; Crystallization; RNA structure; Crystallographic ensembles; Alternate conformation; Long-range motion; Fold and function; Difference Fourier; Non-protein-coding RNA; HEPATITIS-DELTA VIRUS; HEAVY-ATOM DERIVATIVES; RNA HAIRPIN RIBOZYME; FREE R-VALUE; ACTIVE-SITE; DIFFRACTION ANALYSIS; CRYSTAL-STRUCTURE; STRUCTURAL DYNAMICS; TERTIARY STRUCTURE; GENERAL-METHOD;
D O I
10.1016/j.ymeth.2009.06.003
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Relating three-dimensional fold to function is a central challenge in RNA structural biology. Toward this goal, X-ray crystallography has long been considered the "gold standard" for structure determinations at atomic resolution, although NMR spectroscopy has become a powerhouse in this arena as well. In the area of dynamics, NMR remains the dominant technique to probe the magnitude and timescales of molecular motion. Although the latter area remains largely unassailable by conventional crystallographic methods, inroads have been made on proteins using Laue radiation on timescales of ms to ns. Proposed 'fourth generation' radiation sources, such as free-electron X-ray lasers, promise ps- to fs-timescale resolution, and credible evidence is emerging that supports the feasibility of single molecule imaging. At present however, the preponderance of RNA structural information has been derived from timescale and motion insensitive crystallographic techniques. Importantly, developments in computing, automation and high-flux synchrotron sources have propelled the rapidity of 'conventional' RNA crystal structure determinations to timeframes of hours once a suitable set of phases is obtained. With a sufficient number of crystal structures, it is possible to create a structural ensemble that can provide insight into global and local molecular motion characteristics that are relevant to biological function. Here we describe techniques to explore conformational changes in the hairpin ribozyme, a representative non-protein-coding RNA catalyst. The approaches discussed include: (i) construct choice and design using prior knowledge to improve X-ray diffraction; (ii) recognition of long-range conformational changes and (iii) use of single-base or single-atom changes to create ensembles. The methods are broadly applicable to other RNA systems. (c) 2009 Elsevier Inc. All rights reserved.
引用
收藏
页码:87 / 100
页数:14
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