Rapid and reliable RNA resonance assignment by combining chemical and enzymatic stable isotope labeling

IF 2.624
David Klingler , Matthias Huber , Martin Tollinger, Christoph Kreutz
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Abstract

In this work a rapid RNA assignment approach by combining chemical and enzymatic 13C and 15N stable isotope labeling is introduced. We exemplify the assignment strategy for imino N1H1 purine and N3H3 pyrimidine and aromatic C6H6 pyrimidine, C8H8 purine and C2H2 adenine resonances for a non-coding RNA comprising 66 nucleotides. The assignment strategy is based on position specific labeling by chemical solid phase synthesis and dilute stable isotope 13C/15N-labeling by mixing labeled and commercially available unlabeled RNA phosphoramidites. The assignment process is further facilitated by nucleotide specific labeling using T7 RNA polymerase in vitro transcription with in house produced atom specific 13C labeled ribonucleotide triphosphates. The approach is fast with a total NMR measurement time of only 22 h and also competitive in terms of costs as compared to the standard methodology relying on in vitro transcription using 2H, 15N and 13C/15N uniformly labeled ribonucleotide triphosphates. Furthermore, the assignment procedure revealed a slow exchange process on the NMR chemical shift time scale in the 66 nt non-coding RNA with possible biological implications in the regulation of bacterial competence.

Abstract Image

结合化学和酶稳定同位素标记快速可靠的RNA共振分配
本文介绍了一种结合化学和酶的13C和15N稳定同位素标记的快速RNA分配方法。我们举例说明了一个包含66个核苷酸的非编码RNA的亚氨基N1H1嘌呤和N3H3嘧啶以及芳香C6H6嘧啶、C8H8嘌呤和C2H2腺嘌呤共振的分配策略。分配策略是基于化学固相合成的位置特异性标记和稀释稳定同位素13C/ 15n标记,通过混合标记和市售的未标记RNA磷酰胺。使用T7 RNA聚合酶在体外转录中与内部产生的原子特异性13C标记的核糖核苷酸三磷酸进行核苷酸特异性标记,进一步促进了分配过程。该方法快速,总NMR测量时间仅为22小时,与使用2H, 15N和13C/15N均匀标记的核糖核苷酸三磷酸依赖体外转录的标准方法相比,在成本方面也具有竞争力。此外,分配过程揭示了66nt非编码RNA在核磁共振化学位移时间尺度上的缓慢交换过程,这可能在调节细菌能力方面具有生物学意义。
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来源期刊
CiteScore
1.90
自引率
0.00%
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