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Synthesis deprotection analysis and purification of RNA and ribozymes.

机译:RNA和核酶的合成去保护分析和纯化。

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摘要

Improvements in the synthesis, deprotection and purification of oligoribonucleotides are described. These advances allow for reduced synthesis and deprotection times, while improving product yield. Coupling times are reduced by half using 5-ethylthio-1H-tetrazole (S-ethyltetrazole) as the activator. Base and 2'-O-t-butyldimethylsilyl deprotection with methylamine (MA) and anhydrous triethylamine/hydrogen fluoride in N-methylpyrrolidinone (TEA.HF/NMP), respectively, requires a fraction of the time necessitated by current standard methods. In addition, the ease of oligoribonucleotide purification and analysis have been significantly enhanced using anion exchange chromatography. These new methods improve the yield and quality of the oligoribonucleotides synthesized. Hammerhead ribozymes synthesized utilizing the described methods exhibited no diminution in catalytic activity.
机译:描述了寡核糖核苷酸的合成,去保护和纯化的改进。这些进步使得合成和脱保护时间减少,同时提高了产品收率。使用5-乙硫基-1H-四唑(S-乙基四唑)作为活化剂,偶联时间减少一半。在N-甲基吡咯烷酮(TEA.HF / NMP)中分别用甲胺(MA)和无水三乙胺/氟化氢对碱和2'-O-叔丁基二甲基甲硅烷基进行脱保护,所需时间仅是目前标准方法所需时间的一小部分。另外,使用阴离子交换色谱显着提高了寡核糖核苷酸纯化和分析的便利性。这些新方法提高了合成寡核糖核苷酸的产量和质量。利用所述方法合成的锤头状核酶未显示出催化活性的降低。

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