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2
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Metal-ion-dependent folding of a uranyl-specific DNAzyme: insight into function from fluorescence resonance energy transfer studies.金属离子依赖的铀酰特异性 DNA 酶折叠:荧光共振能量转移研究的功能见解。
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Coordination environment of a site-bound metal ion in the hammerhead ribozyme determined by 15N and 2H ESEEM spectroscopy.通过15N和2H电子自旋回波包络调制光谱法测定锤头状核酶中位点结合金属离子的配位环境。
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7
Entropy-driven folding of an RNA helical junction: an isothermal titration calorimetric analysis of the hammerhead ribozyme.RNA螺旋连接的熵驱动折叠:锤头状核酶的等温滴定量热分析
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Folding of the natural hammerhead ribozyme is enhanced by interaction of auxiliary elements.天然锤头状核酶的折叠通过辅助元件的相互作用得以增强。
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9
Cold denaturation of the hammerhead ribozyme.锤头状核酶的冷变性
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10
Dissection of the ion-induced folding of the hammerhead ribozyme using 19F NMR.利用19F核磁共振剖析离子诱导的锤头状核酶折叠过程。
Proc Natl Acad Sci U S A. 2001 May 8;98(10):5503-8. doi: 10.1073/pnas.091097498. Epub 2001 May 1.

离子诱导的锤头状核酶折叠:干扰折叠成活性构象的核心序列变化。

The ion-induced folding of the hammerhead ribozyme: core sequence changes that perturb folding into the active conformation.

作者信息

Bassi G S, Murchie A I, Lilley D M

机构信息

Department of Biochemistry, University, Dundee, United Kingdom.

出版信息

RNA. 1996 Aug;2(8):756-68.

PMID:8752086
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1369413/
Abstract

The hammerhead ribozyme undergoes an ion-dependent folding process into the active conformation. We find that the folding can be blocked at specific stages by changes of sequence or functionality within the core. In the the absence of added metal ions, the global structure of the hammerhead is extended, with a large angle subtended between stems I and II. No core sequence changes appear to alter this geometry, consistent with an unstructured core under these conditions. Upon addition of low concentrations of magnesium ions, the hammerhead folds by an association of stems II and III, to include a large angle between them. This stage is inhibited or altered by mutations within the oligopurine sequence lying between stems II and III, and folding is completely prevented by an A14G mutation. Further increase in magnesium ion concentration brings about a second stage of folding in the natural sequence hammerhead, involving a reorientation of stem I, which rotates around into the same direction of stem II. Because this transition occurs over the same range of magnesium ion concentration over which the hammerhead ribozyme becomes active, it is likely that the final conformation is most closely related to the active form of the structure. Magnesium ion-dependent folding into this conformation is prevented by changes at G5, notably removal of the 2'-hydroxyl group and replacement of the base by cytidine. The ability to dissect the folding process by means of sequence changes suggests that two separate ion-dependent stages are involved in the folding of the hammerhead ribozyme into the active conformation.

摘要

锤头状核酶经历一个离子依赖的折叠过程形成活性构象。我们发现,核心区域内序列或功能的改变可在特定阶段阻断折叠。在没有添加金属离子的情况下,锤头状结构的整体结构是伸展的,茎I和茎II之间形成一个大角度。似乎没有核心序列的变化会改变这种几何结构,这与在这些条件下核心区域无结构的情况一致。加入低浓度的镁离子后,锤头状结构通过茎II和茎III的结合而折叠,它们之间形成一个大角度。茎II和茎III之间的寡嘌呤序列内的突变会抑制或改变这个阶段,而A14G突变则完全阻止折叠。镁离子浓度的进一步增加会使天然序列的锤头状结构进入第二个折叠阶段,涉及茎I的重新定向,它会旋转到与茎II相同的方向。由于这个转变发生在锤头状核酶变得活跃的相同镁离子浓度范围内,最终构象很可能与结构的活性形式关系最为密切。G5处的变化,特别是2'-羟基的去除和碱基被胞嘧啶取代,会阻止镁离子依赖的向这种构象的折叠。通过序列变化剖析折叠过程的能力表明,锤头状核酶折叠成活性构象涉及两个独立的离子依赖阶段。