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首页> 外文期刊>Biochemistry >Mg2+-dependent compaction and folding of yeast tRNAPhe and the catalytic domain of the B. subtilis RNase P RNA determined by small-angle X-ray scattering.
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Mg2+-dependent compaction and folding of yeast tRNAPhe and the catalytic domain of the B. subtilis RNase P RNA determined by small-angle X-ray scattering.

机译:Mg2 +依赖的酵母tRNAPhe的压缩和折叠以及枯草芽孢杆菌RNase P RNA的催化结构域,通过小角度X射线散射测定。

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摘要

We apply synchrotron-based small-angle X-ray scattering to investigate the relationship between compaction, metal binding, and structure formation of two RNAs at 37 degrees C: the 76 nucleotide yeast tRNA(Phe) and the 255 nucleotide catalytic domain of the Bacillus subtilis RNase P RNA. For both RNAs, this method provides direct evidence for the population of a distinct folding intermediate. The relative compaction between the intermediate and the native state does not correlate with the size of the RNA but does correlate well with the amount of surface burial as quantified previously by the urea-dependent m-value. The total compaction process can be described in two major stages. Starting from a completely unfolded state (4-8 M urea, no Mg(2+)), the major amount of compaction occurs upon the dilution of the denaturant and the addition of micromolar amounts of Mg(2+) to form the intermediate. The native state forms in a single transition from the intermediate state upon cooperative binding of three to four Mg(2+) ions. The characterization of this intermediate by small-angle X-ray scattering lends strong support for the cooperative Mg(2+)-binding model to describe the stability of a tertiary RNA.
机译:我们应用基于同步加速器的小角度X射线散射来研究在37°C下两个RNA的紧实,金属结合和结构形成之间的关系:76个核苷酸的酵母tRNA(Phe)和芽孢杆菌的255个核苷酸的催化结构域枯草芽孢杆菌RNase P RNA。对于两种RNA,此方法均可为不同折叠中间体的种群提供直接证据。中间体和天然状态之间的相对紧密性与RNA的大小无关,但与表面掩埋的数量密切相关,如先前由尿素依赖性m值所定量的。整个压实过程可以分为两个主要阶段。从完全展开状态(4-8 M尿素,无Mg(2+))开始,在稀释变性剂和添加微摩尔量的Mg(2+)形成中间体时,发生了大部分压实。原始状态在三到四个Mg(2+)离子的协作结合后从中间状态的单个跃迁中形成。小角度X射线散射对此中间体的表征为描述第三级RNA的稳定性的Mg(2+)结合模型提供了有力的支持。

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