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In-line alignment and Mg2+ coordination at the cleavage site of the env22 twister ribozyme

机译:env22旋绕核酶裂解位点的在线比对和Mg2 +配位

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摘要

Small self-cleaving nucleolytic ribozymes contain catalytic domains that accelerate site-specific cleavage/ligation of phosphodiester backbones. We report on the 2.9-Å crystal structure of the env22 twister ribozyme, which adopts a compact tertiary fold stabilized by co-helical stacking, double-pseudoknot formation and long-range pairing interactions. The U-A cleavage site adopts a splayed-apart conformation with the modeled 2′-O of U positioned for in-line attack on the adjacent to-be-cleaved P-O5′ bond. Both an invariant guanosine and a Mg2+ are directly coordinated to the non-bridging phosphate oxygens at the U-A cleavage step, with the former positioned to contribute to catalysis and the latter to structural integrity. The impact of key mutations on cleavage activity identified an invariant guanosine that contributes to catalysis. Our structure of the in-line aligned env22 twister ribozyme is compared with two recently-reported twister ribozymes structures, which adopt similar global folds, but differ in conformational features around the cleavage site.
机译:小型的自裂解核酶核酶包含催化结构域,可加速磷酸二酯主链的位点特异性裂解/连接。我们报告了env22旋光核酶的2.9-Å晶体结构,该结构采用紧凑的三级折叠结构,该结构通过共螺旋堆积,双假核键形成和远距离配对相互作用而得以稳定。 U-A切割位点采用呈分开的构象,其中U的模型2'-O定位成在线攻击相邻的待切割的P-O5'键。不变的鸟嘌呤和Mg 2 + 在U-A裂解步骤均直接与非桥连的磷酸氧配位,前者有助于催化,后者有助于结构完整性。关键突变对裂解活性的影响确定了不变的鸟苷,有助于催化。我们将在线对齐的env22旋绕核酶的结构与最近报道的两个旋绕核酶结构进行了比较,这两个结构采用相似的整体折叠,但在裂解位点周围的构象特征不同。

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