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Caged circular antisense oligonucleotides for photomodulation of RNA digestion and gene expression in cells

机译:笼状环状反义寡核苷酸,用于光调节RNA消化和细胞中的基因表达

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We synthesized three 20mer caged circular antisense oligodeoxynucleotides (R20, R20B2 and R20B4) with a photocleavable linker and an amide bond linker between two 10mer oligodeoxynucleotides. With these caged circular antisense oligodeoxynucleotides, RNA-binding affinity and its digestion by ribonuclease H were readily photomodulated. RNA cleavage rates were upregulated ~43-, 25- and 15-fold for R20, R20B2 and R20B4, respectively, upon light activation in vitro. R20B2 and R20B4 with 2- or 4-nt gaps in the target RNA lost their ability to bind the target RNA even though a small amount of RNA digestion was still observed. The loss of binding ability indicated promising gene photoregulation through a non-enzymatic strategy. To test this strategy, three caged circular antisense oligonucleotides (PS1, PS2 and PS3) with 2′-OMe RNA and phosphorothioate modifications were synthesized to target GFP expression. Upon light activation, photomodulation of target hybridization and GFP expression in cells was successfully achieved with PS1, PS2 and PS3. These caged circular antisense oligonucleotides show promising applications of photomodulating gene expression through both ribonuclease H and non-enzyme involved antisense strategies.
机译:我们合成了三个20mer笼状环状反义寡聚脱氧核苷酸(R20,R20B2和R20B4),其中两个10mer寡聚脱氧核苷酸之间具有光可裂解的接头和酰胺键接头。利用这些笼状的环状反义寡聚脱氧核苷酸,RNA结合亲和力及其通过核糖核酸酶H的消化容易被光调制。体外光激活后,R20,R20B2和R20B4的RNA裂解率分别上调了约43、25和15倍。尽管仍然观察到少量的RNA消化,但是在靶RNA中具有2或4 nt缺口的R20B2和R20B4失去了结合靶RNA的能力。结合能力的丧失表明通过非酶策略有希望的基因光调节。为了测试该策略,合成了具有2'-OMe RNA和硫代磷酸酯修饰的三个笼状环状反义寡核苷酸(PS1,PS2和PS3)以靶向GFP表达。光激活后,使用PS1,PS2和PS3成功实现了细胞中靶标杂交和GFP表达的光调制。这些笼状的环状反义寡核苷酸显示出通过核糖核酸酶H和涉及非酶的反义策略光调节基因表达的有前途的应用。

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