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Atomic Force Microscopy and Anodic Voltammetry Characterization of a 49-Mer Diels-Alderase Ribozyme

机译:49-Mer Diels-Alderase核酶的原子力显微镜和阳极伏安法表征

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Atomic force microscopy and differential pulse voltammetry were used to characterize the interaction of small highly structured ribozymes with two carbon electrode surfaces. The ribozymes spontaneously self-assemble in two-dimensional networks that cover the entire HOPG surface uniformly. The full-length ribozyme was adsorbed to a lesser extent than a truncated RNA sequence, presumably due to the formation of a more compact overall structure. All four nucleobases composing the ribozyme could be detected by anodic voltammetry on glassy carbon electrodes, and no signals corresponding to free nucleobases were found, indicating the integrity of the ribozyme molecules. Mg~(2+) cations significantly reduced the adsorption of ribozymes to the surfaces, in agreement with the stabilization of this ribozyme's compact, stable, and tightly folded tertiary structure by Mg~(2+) ions that could prevent the hydrophobic bases from interacting with the HOPG surface. Treatment with Pb~(2+) ions, on the other hand, resulted in an increased adsorption of the RNA due to well-known hydrolytic cleavage. The observed dependence of anodic peak currents on different folding states of RNA may provide an attractive method to electrochemically monitor structural changes associated with RNA folding, binding, and catalysis.
机译:原子力显微镜和差分脉冲伏安法用于表征小的高度结构化的核酶与两个碳电极表面的相互作用。核酶自发地自组装成二维网络,均匀覆盖整个HOPG表面。全长核酶的吸附程度比截短的RNA序列小,这可能是由于形成了更紧凑的整体结构所致。组成核酶的所有四个核碱基都可以在玻璃碳电极上通过阳极伏安法检测到,没有发现对应于游离核碱基的信号,表明核酶分子的完整性。 Mg〜(2+)阳离子显着减少了核酶对表面的吸附,这与Mg〜(2+)离子稳定了这种核酶的紧密,稳定和紧密折叠的三级结构相一致,这可以防止疏水性碱基相互作用与HOPG表面。另一方面,由于众所周知的水解裂解,用Pb〜(2+)离子处理导致RNA的吸附增加。观察到的阳极峰值电流对RNA不同折叠状态的依赖性可能为电化学监测与RNA折叠,结合和催化相关的结构变化提供了一种有吸引力的方法。

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