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Rational design of short locked Nucleic Acid-Modified 2′- O -Methyl antisense oligonucleotides for efficient exon-skipping in vitro

机译:短锁核酸修饰的2'-O-甲基反义寡核苷酸的合理设计,可在体外有效跳过外显子

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摘要

Locked nucleic acid is a prominent nucleic acid analog with unprecedented target binding affinity to cDNA and RNA oligonucleotides and shows remarkable stability against nuclease degradation. Incorporation of locked nucleic acid nucleotides into an antisense oligonucleotide (AO) sequence can reduce the length required without compromising the efficacy. In this study, we synthesized a series of systematically truncated locked nucleic acid-modified 2′-O-methyl AOs on a phosphorothioate (PS) backbone that were designed to induce skipping exon 23 from the dystrophin transcript in H-2Kb-tsA58 mdx mouse myotubes in vitro. The results clearly demonstrated that shorter AOs (16- to 14-mer) containing locked nucleic acid nucleotides efficiently induced dystrophin exon 23 skipping compared with the corresponding 2′-O-methyl AOs. Our remarkable findings contribute significantly to the existing knowledge about the designing of short LNA-modified oligonucleotides for exon-skipping applications, which will help reduce the cost of exon-skipping AOs and potential toxicities, particularly the 2′-OMe-based oligos, by further reducing the length of AOs.
机译:锁定核酸是一种杰出的核酸类似物,对cDNA和RNA寡核苷酸具有空前的靶结合亲和力,并且显示出显着的抗核酸酶降解稳定性。将锁定的核酸核苷酸掺入反义寡核苷酸(AO)序列中可以减少所需的长度,而不损害功效。在这项研究中,我们在硫代磷酸酯(PS)骨架上合成了一系列系统地截短的,被锁定的,核酸修饰的2'-O-甲基AO,旨在诱导H-2Kb-tsA58 mdx小鼠的肌营养不良蛋白转录本跳过外显子23体外肌管。结果清楚地表明,与相应的2'-O-甲基AO相比,包含锁定核酸核苷酸的较短AO(16至14-mer)可有效诱导肌营养不良蛋白外显子23跳跃。我们的杰出发现为现有的有关设计短LNA修饰寡核苷酸以用于外显子跳跃应用的知识做出了重要贡献,这将有助于降低外显子跳跃AO的成本和潜在的毒性,特别是通过2'-OMe修饰的寡核苷酸。进一步减少了AO的长度。

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