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Kinetics of tRNA folding monitored by aminoacylation

机译:通过氨酰化监测tRNA折叠的动力学

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摘要

We describe a strategy for tracking Mg2+-initiated folding of 32P-labeled tRNA molecules to their native structures based on the capacity for aminoacylation by the cognate aminoacyl-tRNA synthetase enzyme. The approach directly links folding to function, paralleling a common strategy used to study the folding of catalytic RNAs. Incubation of unfolded tRNA with magnesium ions, followed by the addition of aminoacyl-tRNA synthetase and further incubation, yields a rapid burst of aminoacyl-tRNA formation corresponding to the prefolded tRNA fraction. A subsequent slower increase in product formation monitors continued folding in the presence of the enzyme. Further analysis reveals the presence of a parallel fraction of tRNA that folds more rapidly than the majority of the population. The application of the approach to study the influence of post-transcriptional modifications in folding of Escherichia coli tRNA1Gln reveals that the modified bases increase the folding rate but do not affect either the equilibrium between properly folded and misfolded states or the folding pathway. This assay allows the use of 32P-labeled tRNA in integrated studies combining folding, post-transcriptional processing, and aminoacylation reactions.
机译:我们描述了一种策略,该方法基于同源氨基酰-tRNA合成酶的氨酰化能力,跟踪由Mg 2 + 引发的 32 P标记的tRNA分子折叠至其天然结构酶。该方法直接将折叠与功能联系起来,与用于研究催化性RNA折叠的常用策略相平行。将未折叠的tRNA与镁离子一起孵育,然后添加氨酰基-tRNA合成酶并进一步温育,从而产生与预折叠的tRNA馏分相对应的氨酰基-tRNA形成快速爆发。在酶的存在下,随后产物形成的缓慢增加监测了连续折叠。进一步的分析表明,存在平行的tRNA部分,其折叠速度比大多数人群快。该方法在研究转录后修饰对大肠杆菌tRNA1 Gln 折叠的影响中的应用表明,修饰的碱基可提高折叠速率,但不会影响正确折叠和错误折叠状态之间的平衡或折叠路径。该测定法允许在结合折叠,转录后加工和氨基酰化反应的综合研究中使用 32 P标记的tRNA。

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