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Preparation and characterization of a uniformly 2 H/ 15 N-labeled RNA oligonucleotide for NMR studies.

机译:用于NMR研究的均匀2 H / 15 N标记的RNA寡核苷酸的制备和表征。

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摘要

An RNA oligonucleotide that contains the binding site for Escherichia coli ribosomal protein S8 was prepared with uniform 15N isotopic enrichment and uniform deuterium enrichment at all non-exchangeable sites using enzymatic methods. The RNA binding site, which contains 44 nt, forms a hairpin in solution and requires Mg2+for proper folding. The longitudinal magnetization recovery rates of the exchangeable protons were compared for the [2H,15N]-enriched RNA molecule and for the corresponding fully [2H,15N]-enriched RNA hairpin. It was found that 1H-1H dipolar relaxation significantly contributes to the recovery of exchangeable proton longitudinal magnetization. The exchangeable proton resonance line widths were less affected by deuteration, indicating that chemical exchange with H2O remains the dominant mechanism of transverse magnetization relaxation. Nevertheless, deuteration of this RNA hairpin was found to enhance the sensitivity of NOE-based experiments relative to the fully protonated hairpin and to simplify 2D NMR spectra. The increased signal-to-noise ratio facilitated the assignment of the cytidine amino resonances and several of the purine nucleotide amino resonances and permitted the identification of NOE crosspeaks that could not be observed in spectra of the fully protonated RNA hairpin.
机译:使用酶促方法制备了包含大肠杆菌核糖体蛋白S8结合位点的RNA寡核苷酸,在所有不可交换的位点均具有均匀的15N同位素富集和氘重均富集。 RNA结合位点包含44 nt,在溶液中形成发夹,需要Mg2 +才能正确折叠。比较了[2H,15N]富集的RNA分子和相应的[2H,15N]富集的RNA发夹的可交换质子的纵向磁化恢复率。发现1H-1H偶极弛豫显着有助于可交换质子纵向磁化的恢复。可交换质子共振线的宽度受氘的影响较小,表明与H2O的化学交换仍然是横向磁化弛豫的主要机制。尽管如此,发现这种RNA发夹的氘化相对于完全质子化的发夹增强了基于NOE的实验的灵敏度,并简化了2D NMR光谱。信噪比的增加促进了胞苷氨基共振和一些嘌呤核苷酸氨基共振的分配,并允许鉴定在完全质子化的RNA发夹的光谱中无法观察到的NOE交叉峰。

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