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Molecular modelling of the GIR1 branching ribozyme gives new insight into evolution of structurally related ribozymes

机译:GIR1分支核酶的分子模型为结构相关核酶的进化提供了新见解

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摘要

Twin-ribozyme introns contain a branching ribozyme (GIR1) followed by a homing endonuclease (HE) encoding sequence embedded in a peripheral domain of a group I splicing ribozyme (GIR2). GIR1 catalyses the formation of a lariat with 3 nt in the loop, which caps the HE mRNA. GIR1 is structurally related to group I ribozymes raising the question about how two closely related ribozymes can carry out very different reactions. Modelling of GIR1 based on new biochemical and mutational data shows an extended substrate domain containing a GoU pair distinct from the nucleophilic residue that dock onto a catalytic core showing a different topology from that of group I ribozymes. The differences include a core J8/7 region that has been reduced and is complemented by residues from the pre-lariat fold. These findings provide the basis for an evolutionary mechanism that accounts for the change from group I splicing ribozyme to the branching GIR1 architecture. Such an evolutionary mechanism can be applied to other large RNAs such as the ribonuclease P.
机译:双核酶内含子包含一个分支核酶(GIR1),随后是一个归巢于核酸内切酶(HE)的编码序列,该编码序列嵌入在I组剪接核酶(GIR2)的外围结构域中。 GIR1催化环中3 nt的套索的形成,该套帽覆盖了HE mRNA。 GIR1在结构上与第I组核酶有关,从而提出了一个问题,即两个密切相关的核酶如何进行截然不同的反应。基于新的生化和突变数据对GIR1的建模显示了一个扩展的底物结构域,该结构域包含一个GoU对,该GoU对不同于对接至催化核心的亲核残基,显示出与I类核酶不同的拓扑。差异包括核心J8 / 7区,该区已被还原,并由lariat折叠前的残基补充。这些发现为进化机制奠定了基础,该机制解释了从I组剪接核酶到分支GIR1结构的变化。这样的进化机制可以应用于其他大RNA,例如核糖核酸酶P。

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