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Exploring TAR-RNA aptamer loop-loop interaction by X-ray crystallography, UV spectroscopy and surface plasmon resonance

机译:通过X射线晶体学,UV光谱和表面等离子体共振研究TAR-RNA适体环-环相互作用

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In HIV-1, trans-activation of transcription of the viral genome is regulated by an imperfect hairpin, the trans-activating responsive (TAR) RNA element, located at the 5' untranslated end of all viral transcripts. TAR acts as a binding site for viral and cellular proteins. In an attempt to identify RNA ligands that would interfere with the virus life-cycle by interacting with TAR, an in vitro selection was previously carried out. RNA hairpins that formed kissing-loop dimers with TAR were selected [Duconge F. and Toulme JJ (1999) RNA, 5:1605-1614]. We describe here the crystal structure of TAR bound to a high-affinity RNA aptamer. The two hairpins form a kissing complex and interact through six Watson-Crick base pairs. The complex adopts an overall conformation with an inter-helix angle of 28.1 degrees , thus contrasting with previously reported solution and modelling studies. Structural analysis reveals that inter-backbone hydrogen bonds between ribose 2' hydroxyl and phosphate oxygens at the stem-loop junctions can be formed. Thermal denaturation and surface plasmon resonance experiments with chemically modified 2'-O-methyl incorporated into both hairpins at key positions, clearly demonstrate the involvement of this intermolecular network of hydrogen bonds in complex stability.
机译:在HIV-1中,病毒基因组转录的反式激活受不完善的发夹的调节,该发夹位于所有病毒转录本的5'非翻译末端的反式激活响应(TAR)RNA元件。 TAR充当病毒和细胞蛋白的结合位点。为了鉴定通过与TAR相互作用会干扰病毒生命周期的RNA配体,先前进行了体外选择。选择与TAR形成亲吻环二聚体的RNA发夹[Duconge F.和Toulme JJ(1999)RNA,5:1605-1614]。我们在这里描述TAR的晶体结构绑定到高亲和性RNA适体。两个发夹形成一个接吻复合体,并通过六个Watson-Crick碱基对相互作用。该复合物采用整体构型,螺旋间角为28.1度,因此与先前报道的解决方案和模型研究形成了对比。结构分析表明,可以在茎-环连接处形成核糖2'羟基和磷酸氧之间的骨干间氢键。将化学修饰的2'-O-甲基并入两个发夹的关键位置进行的热变性和表面等离振子共振实验清楚地证明了这种氢键分子间网络参与了复杂的稳定性。

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