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Post-crystallization Improvement of RNA Crystals by Synergistic Ion Exchange and Dehydration

机译:协同离子交换和脱水作用改善RNA晶体的后结晶

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摘要

Compared to the recent dramatic growth in the numbers of genome-wide and functional studies of complex non-coding RNAs, mechanistic and structural analyses have lagged behind. A major technical bottleneck in the structural determination of large RNAs and their complexes is preparation of diffracting crystals. Empirically, a vast majority of such RNA crystals fail to diffract X-rays to usable resolution (~4 Å) due to their inherent disorder and non-specific packing within the crystals. Here, we present a protocol that combines post-crystallization cation replacement and dehydration that dramatically improved the diffraction quality of crystals of a large gene-regulatory mRNA-tRNA complex. This procedure not only extended the resolution limit of X-ray data from 8.5 to 3.2 Å, but also significantly improved the quality of the data, enabling de novo phasing and structure determination. Because it exploits the general importance of counterions and solvation in RNA structure, this procedure may prove broadly useful in the crystallographic analyses of other large non-coding RNAs.
机译:与最近对复杂的非编码RNA进行全基因组和功能研究的数量急剧增加相比,机械和结构分析滞后了。大RNA及其复合物结构测定中的主要技术瓶颈是衍射晶体的制备。根据经验,绝大多数此类RNA晶体由于其固有的无序性和晶体内的非特异性堆积而无法将X射线衍射至可用分辨率(〜4Å)。在这里,我们提出了一种结合了结晶后阳离子置换和脱水的协议,该协议可以显着提高大型基因调节mRNA-tRNA复合物晶体的衍射质量。此过程不仅将X射线数据的分辨率限制从8.5扩展到3.2Å,而且还显着提高了数据质量,从而可以从头定相并确定结构。因为它利用了抗衡离子和溶剂化在RNA结构中的一般重要性,所以该方法可能在其他大型非编码RNA的晶体学分析中被广泛使用。

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