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Combining asymmetric C-13-labeling and isotopic filter/edit NOESY: a novel strategy for rapid and logical RNA resonance assignment

机译:结合不对称C-13标记和同位素过滤器/编辑Noesy:一种新的快速和逻辑RNA共振分配策略

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摘要

Although similar to 98% of the human genomic output is transcribed as non-protein coding RNA, < 2% of the protein data bank structures comprise RNA. This huge structural disparity stems from combined difficulties of crystallizing RNA for X-ray crystallography along with extensive chemical shift overlap and broadened linewidths associated with NMR of RNA. While half of the deposited RNA structures in the PDB were solved by NMR methods, the usefulness of NMR is still limited by the high cost of sample preparation and challenges of resonance assignment. Here we propose a novel strategy for resonance assignment that combines new strategic C-13 labeling technologies with filter/ edit type NOESY experiments to greatly reduce spectral complexity and crowding. This new strategy allowed us to assign important non-exchangeable resonances of proton and carbon (1', 2', 2, 5, 6 and 8) nuclei using only one sample and < 24 h of NMR instrument time for a 27 nt model RNA. The method was further extended to assigning a 6 nt bulge froma 61 nt viral RNA element justifying its use for a wide range RNA chemical shift resonance assignment problems.
机译:尽管与非蛋白质编码RNA类似于98%的人类基因组输出,但蛋白质数据群结构的<2%包括RNA。这种巨大的结构视差源于结晶RNA的X射线晶体学的结晶困难以及广泛的化学换档重叠和与RNA NMR相关的宽度。虽然通过NMR方法解决了PDB中的一半沉积的RNA结构,但NMR的有用性仍然受到样品制备的高成本和共振分配的挑战的限制。在这里,我们提出了一种新的共振转让策略,将新的战略C-13标记技术与过滤器/编辑类型Noesy实验相结合,大大降低了光谱复杂性和拥挤。这种新策略使我们可以使用仅使用一个样品和24小时的NMR仪器时间来分配质子和碳(1',2',2,2,5,6和8)核的重要不可交换的共振27 nt模型RNA 。该方法进一步扩展为分配6nt凸出从61nt病毒RNA元素,证明其用于宽范围的RNA化学换档共振分配问题。

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