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Biochemical detection of monovalent metal ion binding sites within RNA.

机译:RNA中单价金属离子结合位点的生化检测。

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摘要

Many RNAs, including the ribosome, RNase P, and the group II intron, explicitly require monovalent cations for activity in vitro. Although the necessity of monovalent cations for RNA function has been known for more than a quarter of a century, the characterization of specific monovalent metal sites within large RNAs has been elusive. Here we describe a biochemical approach to identify functionally important monovalent cations in nucleic acids. This method uses thallium (Tl+), a soft Lewis acid heavy metal cation with chemical properties similar to those of the physiological alkaline earth metal potassium (K+). Nucleotide analog interference mapping (NAIM) with the sulfur-substituted nucleotide 6-thioguanosine in combination with selective metal rescue of the interference with Tl+ provides a distinct biochemical signature for monovalent metal ion binding. This approach has identified a K+ binding site within the P4-P6 domain of the Tetrahymena group I intron that is also present within the X-ray crystal structure. The technique also predicted a similar binding site within the Azoarcus group I intron where the structure is not known. The approach is applicable to any RNA molecule that can be transcribed in vitro and whose function can be assayed.
机译:许多RNA,包括核糖体,RNase P和II组内含子,明确要求单价阳离子具有体外活性。尽管已知四价阳离子具有RNA功能的必要性已超过四分之一世纪,但对大型RNA中特定单价金属位点的表征却难以捉摸。在这里,我们描述了一种生物化学方法来鉴定核酸中功能上重要的单价阳离子。该方法使用th(Tl +),一种软路易斯酸重金属阳离子,其化学性质与生理碱土金属钾(K +)相似。具有硫取代的核苷酸6-硫代鸟苷的核苷酸类似物干扰图谱(NAIM)与对Tl +的干扰的选择性金属挽救相结合,为单价金属离子结合提供了独特的生化特征。该方法已经鉴定了四膜虫群I内含子的P4-P6结构域内的K +结合位点,其也存在于X射线晶体结构内。该技术还预测了偶氮第一类内含子内含子的相似结合位点,该结构未知。该方法适用于可在体外转录且可测定其功能的任何RNA分子。

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