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The 1.4-Å crystal structure of the S. pombe Pop2p deadenylase subunit unveils the configuration of an active enzyme

机译:粟酒裂殖酵母Pop2p腺苷酸酶亚基的1.4-Å晶体结构揭示了活性酶的构型

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摘要

Deadenylation is the first and probably also rate-limiting step of controlled mRNA decay in eukaryotes and therefore central for the overall rate of gene expression. In yeast, the process is maintained by the mega-Dalton Ccr4-Not complex, of which both the Ccr4p and Pop2p subunits are 3′–5′ exonucleases potentially responsible for the deadenylation reaction. Here, we present the crystal structure of the Pop2p subunit from Schizosaccharomyces pombe determined to 1.4 Å resolution and show that the enzyme is a competent ribonuclease with a tunable specificity towards poly-A. In contrast to S. cerevisiae Pop2p, the S. pombe enzyme contains a fully conserved DEDDh active site, and the high resolution allows for a detailed analysis of its configuration, including divalent metal ion binding. Functional data further indicates that the identity of the ions in the active site can modulate both activity and specificity of the enzyme, and finally structural superposition of single nucleotides and poly-A oligonucleotides provide insight into the catalytic cycle of the protein.
机译:腺苷酸化是真核生物中受控mRNA衰变的第一步,也是可能的限速步骤,因此对于基因表达的整体速率至关重要。在酵母中,该过程由巨型道尔顿Ccr4-Not复合物维持,该复合物的Ccr4p和Pop2p亚基均为3'–5'核酸外切酶,可能引起死烯化反应。在这里,我们介绍了来自粟酒裂殖酵母的Pop2p亚基的晶体结构,已确定其分辨率为1.4resolutionÅ,并表明该酶是一种有能力的核糖核酸酶,对poly-A具有可调的特异性。与酿酒酵母Pop2p相比,粟酒裂殖酵母酶包含一个完全保守的DEDDh活性位点,并且高分辨率允许对其构型进行详细分析,包括二价金属离子结合。功能数据进一步表明,活性位点中离子的身份可以调节酶的活性和特异性,最后单核苷酸和聚A寡核苷酸的结构叠加为深入了解蛋白质的催化循环提供了条件。

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