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Enzymatic incorporation of an azide-modified UTP analog into oligoribonucleotides for post-transcriptional chemical functionalization

机译:将叠氮化物修饰的UTP类似物酶促整合到寡核糖核苷酸中以进行转录后化学功能化

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摘要

This protocol describes the detailed experimental procedure for the synthesis of an azide-modified uridine triphosphate analog and its effective incorporation into an oligoribonucleotide by in vitro transcription reactions. Furthermore, procedures for labeling azide-modified oligoribonucleotides post-transcriptionally with biophysical probes by copper(I)-catalyzed alkyne-azide cycloaddition (CuAAC) and Staudinger reactions are also provided. This post-transcriptional chemical modification protocol is simple and modular, and it affords labeled oligonucleotides in reasonable amounts for biophysical assays. The procedure for enzymatic incorporation of the monophosphate of azide-modified UTP into an oligoribonucleotide transcript takes ~2 d, and subsequent post-transcriptional chemical functionalization of the transcript takes about 2 d.
机译:该协议描述了叠氮化物修饰的尿苷三磷酸类似物的合成及其通过体外转录反应有效掺入寡核糖核苷酸的详细实验程序。此外,还提供了通过铜(I)催化的炔-叠氮化物环加成(CuAAC)和施陶丁格反应用生物物理探针在转录后标记叠氮化物修饰的寡核糖核苷酸的步骤。该转录后化学修饰方案简单,模块化,可提供合理数量的标记寡核苷酸用于生物物理测定。将叠氮化物修饰的UTP的单磷酸酶促掺入寡核糖核苷酸转录物中的过程约需2 d,随后转录本的转录后化学功能化约需2 d。

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