Application of RtcB ligase to monitor self-cleaving ribozyme activity by RNA-seq

核酶 连接酶核酶 RNA连接酶 DNA连接酶 核糖核酸 适配器(计算) 核酶 化学 结扎 生物化学 发夹状核酶 哺乳动物CPEB3核酶 分子生物学 DNA 计算生物学 生物 基因 计算机科学 操作系统
作者
V Janett Olzog,Lena I. Freist,Robin Goldmann,Jörg Fallmann,Christina E. Weinberg
出处
期刊:Biological Chemistry [De Gruyter]
卷期号:403 (8-9): 705-715 被引量:3
标识
DOI:10.1515/hsz-2021-0408
摘要

Abstract Self-cleaving ribozymes are catalytic RNAs and can be found in all domains of life. They catalyze a site-specific cleavage that results in a 5′ fragment with a 2′,3′ cyclic phosphate (2′,3′ cP) and a 3′ fragment with a 5′ hydroxyl (5′ OH) end. Recently, several strategies to enrich self-cleaving ribozymes by targeted biochemical methods have been introduced by us and others. Here, we develop an alternative strategy in which 5ʹ OH RNAs are specifically ligated by RtcB ligase, which first guanylates the 3′ phosphate of the adapter and then ligates it directly to RNAs with 5′ OH ends. Our results demonstrate that adapter ligation to highly structured ribozyme fragments is much more efficient using the thermostable RtcB ligase from Pyrococcus horikoshii than the broadly applied Escherichia coli enzyme. Moreover, we investigated DNA, RNA and modified RNA adapters for their suitability in RtcB ligation reactions. We used the optimized RtcB-mediated ligation to produce RNA-seq libraries and captured a spiked 3ʹ twister ribozyme fragment from E. coli total RNA. This RNA-seq-based method is applicable to detect ribozyme fragments as well as other cellular RNAs with 5ʹ OH termini from total RNA.
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