4′-C-Acetamidomethyl-2′-O-methoxyethyl Nucleic Acid Modifications Improve Thermal Stability, Nuclease Resistance, Potency, and hAgo2 Binding of Small Interfering RNAs

核酸酶 核酸 基因沉默 寡核苷酸 胸苷 化学 热稳定性 尿苷 小干扰RNA 复式(建筑) 分子生物学 立体化学 生物化学 DNA 核糖核酸 基因 生物 有机化学
作者
Sumit Gangopadhyay,Gautam Das,Shalini Gupta,Atanu Ghosh,Siddharam Shivappa Bagale,Pritam Roy,Mahitosh Mandal,S. Harikrishna,Surajit Sinha,Kiran R. Gore
出处
期刊:Journal of Organic Chemistry [American Chemical Society]
卷期号:89 (6): 3747-3768
标识
DOI:10.1021/acs.joc.3c02506
摘要

In this study, we designed the 4′-C-acetamidomethyl-2′-O-methoxyethyl (4′-C-ACM-2′-O-MOE) uridine and thymidine modifications, aiming to test them into small interfering RNAs. Thermal melting studies revealed that incorporating a single 4′-C-ACM-2′-O-MOE modification in the DNA duplex reduced thermal stability. In contrast, an increase in thermal stability was observed when the modification was introduced in DNA:RNA hybrid and in siRNAs. Thermal destabilization in DNA duplex was attributed to unfavorable entropy, which was mainly compensated by the enthalpy factor to some extent. A single 4′-C-ACM-2′-O-MOE thymidine modification at the penultimate position of the 3′-end of dT20 oligonucleotides in the presence of 3′-specific exonucleases, snake venom phosphodiesterase (SVPD), demonstrated significant stability as compared to monomer modifications including 2′-O-Me, 2′-O-MOE, and 2′-F. In gene silencing studies, we found that the 4′-C-ACM-2′-O-MOE uridine or thymidine modifications at the 3′-overhang in the passenger strand in combination with two 2′-F modifications exhibited superior RNAi activity. The results suggest that the dual modification is well tolerated at the 3′-end of the passenger strand, which reflects better siRNA stability and silencing activity. Interestingly, 4′-C-ACM-2′-O-MOE-modified siRNAs showed considerable gene silencing even after 96 h posttransfection; it showed that our modification could induce prolonged gene silencing due to improved metabolic stability. Molecular modeling studies revealed that the introduction of the 4′-C-ACM-2′-O-MOE modification at the 3′-end of the siRNA guide strand helps to anchor the strand within the PAZ domain of the hAgo2 protein. The overall results indicate that the 4′-C-ACM-2′-O-MOE uridine and thymidine modifications are promising modifications to improve the stability, potency, and hAgo2 binding of siRNAs.
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