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首页> 外文期刊>Nucleic Acids Research >LNA/DNA chimeric oligomers mimic RNA aptamers targeted to the TAR RNA element of HIV-1
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LNA/DNA chimeric oligomers mimic RNA aptamers targeted to the TAR RNA element of HIV-1

机译:LNA / DNA嵌合低聚物模拟针对HIV-1的TAR RNA元件的RNA适体

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摘要

One of the major limitations of the use of phosphodiester oligonucleotides in cells is their rapid degradation by nucleases. To date, several chemical modifications have been employed to overcome this issue but insufficient efficacy and/or specificity have limited their in vivo usefulness. In this work conformationally restricted nucleotides, locked nucleic acid (LNA), were investigated to design nuclease resistant aptamers targeted against the HIV-1 TAR RNA. LNA/DNA chimeras were synthesized from a shortened version of the hairpin RNA aptamer identified by in vitro selection against TAR. The results indicate that these modifications confer good protection towards nuclease digestion. Electrophoretic mobility shift assays, thermal denaturation monitored by UV-spectroscopy and surface plasmon resonance experiments identified LNA/DNA TAR ligands that bind to TAR with a dissociation constant in the low nanomolar range as the parent RNA aptamer. The crucial G, A residues that close the aptamer loop remain a key structural determinant for stable LNA/DNA chimera–TAR complexes. This work provides evidence that LNA modifications alternated with DNA can generate stable structured RNA mimics for interacting with folded RNA targets.
机译:在细胞中使用磷酸二酯寡核苷酸的主要限制之一是它们被核酸酶快速降解。迄今为止,已经采用了几种化学修饰来克服该问题,但是功效和/或特异性不足限制了它们的体内实用性。在这项工作中,对构象受限的核苷酸锁核酸(LNA)进行了研究,以设计针对HIV-1 TAR RNA的核酸酶抗性适体。 LNA / DNA嵌合体由发夹RNA适体的缩短版本合成,该发夹RNA适体通过针对TAR的体外选择而鉴定。结果表明,这些修饰赋予了对核酸酶消化的良好保护。电泳迁移率变化分析,通过紫外光谱监测的热变性和表面等离子体共振实验确定了以低纳摩尔范围的解离常数与TAR结合的LNA / DNA TAR配体作为母体RNA适体。封闭适体环的关键G,A残基仍然是稳定LNA / DNA嵌合体– TAR复合物的关键结构决定因素。这项工作提供了证据,证明LNA修饰与DNA交替可以产生稳定的结构化RNA模拟物,以与折叠的RNA靶标相互作用。

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