Photomodulating RNA cleavage using photolabile circular antisense oligodeoxynucleotides

劈理(地质) 寡核苷酸 核酸 磷酰胺 核酸酶 反义RNA 生物化学 碱基对 抄写(语言学) 核酸内切酶 转移RNA 翻译(生物学) RNA依赖性RNA聚合酶
作者
Xinjing Tang,Meng Su,Lili Yu,Cong Lv,Jie Wang,Zhongjin Li
出处
期刊:Nucleic Acids Research [Oxford University Press]
卷期号:38 (11): 3848-3855 被引量:45
标识
DOI:10.1093/nar/gkq079
摘要

Caged antisense oligodeoxynucleotides (asODNs) are synthesized by linking two ends of linear oligodeoxynucleotides using a photocleavable linker. Two of them (H30 and H40) have hairpin-like structures which show a large difference in thermal stability (Delta T(m) = 17.5 degrees C and 11.6 degrees C) comparing to uncaged ones. The other three (C20, C30 and C40) without stable secondary structures have the middle 20 deoxynucleotides complementary to 40-mer RNA. All caged asODNs have restricted opening which provides control over RNA/asODN interaction. RNase H assay results showed that 40-mer RNA digestion could be photo-modulated 2- to 3-fold upon light-activation with H30, H40, C30 and C40, while with C20, RNA digestion was almost not detectable; however, photo-activation triggered >20-fold increase of RNA digestion. And gel shift assays showed that it needed >0.04 microM H40 and 0.5 microM H30 to completely bind 0.02 microM 40-mer RNA, and for C40 and C30, it needed >0.2 microM and 0.5 microM for 0.02 microM 40-mer RNA binding. However, even 4 microM C20 was not able to fully bind the same concentration of 40-mer RNA. By simple adjustment of ring size of caged asODNs, we could successfully photoregulate their hybridization with mRNA and target RNA hydrolysis by RNase H with light activation.

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