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Mg2+-dependent folding of a Diels-Alderase ribozyme probed by single-molecule FRET analysis

机译:通过单分子FRET分析探测Diels-Alderase核酶的Mg2 +依赖性折叠

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Here, we report a single-molecule fluorescence resonance energy transfer (FRET) study of a Diels-Alderase (DAse) ribozyme, a 49-mer RNA with true catalytic properties. The DAse ribozyme was labeled with Cy3 and Cy5 as a FRET pair of dyes to observe intramolecular folding, which is a prerequisite for its recognition and turnover of two organic substrate molecules. FRET efficiency histograms and kinetic data were taken on a large number of surface-immobilized ribozyme molecules as a function of the Mg2+ concentration in the buffer solution. From these data, three separate states of the DAse ribozyme can be distinguished, the unfolded (U), intermediate (I) and folded (F) states. A thermodynamic model was developed to quantitatively analyze the dependence of these states on the Mg2+ concentration. The FRET data also provide information on structural properties. The I state shows a strongly cooperative compaction with increasing Mg2+ concentration that arises from association with several Mg2+ ions. This transition is followed by a second Mg2+-dependent cooperative transition to the F state. The observation of conformational heterogeneity and continuous fluctuations between the I and F states on the ~100?ms timescale offers insight into the folding dynamics of this ribozyme.
机译:在这里,我们报告Diels-醛糖酶(DAse)核酶,具有真正催化特性的49-mer RNA的单分子荧光共振能量转移(FRET)研究。 DAse核酶用Cy3和Cy5标记为FRET对染料,以观察分子内折叠,这是其识别和转换两个有机底物分子的前提。根据大量固定在表面上的核酶分子的FRET效率直方图和动力学数据,作为缓冲溶液中Mg 2 + 浓度的函数。根据这些数据,可以区分DAse核酶的三个独立状态,即未折叠(U),中间(I)和折叠(F)状态。建立了一个热力学模型来定量分析这些状态对Mg 2 + 浓度的依赖性。 FRET数据还提供有关结构特性的信息。 I状态显示出随着与几个Mg 2 + 离子缔合而产生的Mg 2 + 浓度增加的强烈协同压缩作用。该转变之后是第二个依赖于Mg 2 + 的协同转变为F状态。在〜100?ms时间尺度上观察到构象异质性和I和F状态之间的连续波动,可以深入了解这种核酶的折叠动力学。

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