Direct dsRNA preparation by promoter-free RCT and RNase H cleavage using one circular dsDNA template with a mismatched bubble

RNA沉默 生物 核糖核酸 T7 RNA聚合酶 核糖核酸酶P 抄写(语言学) RNA聚合酶 核糖核酸酶H RNA依赖性RNA聚合酶 分子生物学 聚合酶 RNA干扰 DNA 遗传学 基因 噬菌体 大肠杆菌 语言学 哲学
作者
Hui Chen,Zongchao Gu,Yang Liu,Feng Li,Ran An,Yubin Ge,Xingguo Liang
出处
期刊:RNA [Cold Spring Harbor Laboratory Press]
卷期号:29 (11): 1691-1702
标识
DOI:10.1261/rna.079670.123
摘要

Double-stranded RNA (dsRNA) has aroused widespread interest due to its effects on immunity and applications based on RNAi. However, the in vitro preparation of dsRNA is costly and laborious. In this study, we have developed a novel and interesting method designated as pfRCT (promoter-free rolling-circle transcription) for direct, facile, and efficient dsRNA preparation. This method generates equal amounts of sense and antisense strands simultaneously from a single circular dsDNA template. To initiate transcription by T7 RNA polymerase without directional preference, a 9-15-bp bubble (mismatched duplex with strong sequence symmetry) is introduced into the template. During RCT, all the necessary reagents, including the template, NTPs, RNA polymerase, RNase H, and Helpers, are present in one pot; and the just-transcribed RNA is immediately truncated by RNase H to monomers with the desired size. The ends of the dsRNA product can also be simply sealed by T4 RNA ligase 1 after pfRCT. This new approach is expected to promote the applications of dsRNA.
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