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A robust and versatile method for production and purification of large-scale RNA samples for structural biology

机译:一种稳健且多功能的方法用于生产和纯化大型RNA样品的结构生物学

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摘要

Recent findings in genome-wide transcriptomics revealed that RNAs are involved in almost every biological process, across all domains of life. The characterization of native RNAs of unknown function and structure is particularly challenging due to their typical low abundance in the cell and the inherent sensitivity toward ubiquitous RNA degrading enzymes. Therefore, robust in vitro synthesis and extensive work-up methods are often needed to obtain samples amenable for biochemical, biophysical, and structural studies. Here, we present a protocol that combines the most recent advances in T7 in vitro transcription methodology with reverse phase ion pairing and ion exchange HPLC purification of RNAs for the production of yield-optimized large-scale samples. The method is easy to follow, robust and suitable for users with little or no experience within the field of biochemistry or chromatography. The complete execution of this method, for example, for production of isotopically labeled NMR samples, can be performed in less than a week.
机译:最近在基因组转录组织中的发现显示,RNA几乎涉及所有生命域的生物过程。由于其细胞中典型的低丰度以及对普遍存在RNA降解酶的固有敏感性,未知功能和结构的天然RNA的表征尤其具有挑战性。因此,通常需要稳健的体外合成和广泛的后处理方法,以获得适用于生物化学,生物物理和结构研究的样品。在这里,我们提出了一种协议,其将T7体外转录方法中的最新进展与RNA的反相离子配对和离子交换HPLC纯化结合在于生产产量优化的大规模样品。该方法易于遵循,强大,适用于生物化学或色谱结构少或没有经验的用户。例如,用于生产同位素标记的NMR样品的方法,可以在不到一周内进行该方法。

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