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The active site architecture of Pisum sativum β-carbonic anhydrase is a mirror image of that of α-carbonic anhydrases

机译:豌豆(Pisum sativum)β-碳酸酐酶的活性位点结构与α-碳酸酐酶的活性位点镜像

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摘要

We have determined the structure of the β–carbonic anhydrase from the dicotyledonous plant Pisum sativum at 1.93 Å resolution, using a combination of multiple anomalous scattering off the active site zinc ion and non-crystallographic symmetry averaging. The mol– ecule assembles as an octamer with a novel dimer of dimers of dimers arrangement. Two distinct patterns of conservation of active site residues are observed, implying two potentially mechanistically distinct classes of β–carbonic anhydrases. The active site is located at the interface between two monomers, with Cys160, His220 and Cys223 binding the catalytic zinc ion and residues Asp162 (oriented by Arg164), Gly224, Gln151, Val184, Phe179 and Tyr205 interacting with the substrate analogue, acetic acid. The substrate binding groups have a one to one correspondence with the functional groups in the α–carbonic anhydrase active site, with the corresponding residues being closely superimposable by a mirror plane. Therefore, despite differing folds, α- and β–carbonic anhydrase have converged upon a very similar active site design and are likely to share a common mechanism.
机译:我们结合活性位点锌离子的多个异常散射和平均非晶体对称性,确定了双子叶植物Pisum sativum的β-碳酸酐酶的结构,分辨率为1.93 93。分子以八聚体形式与新型的二聚体二聚体组装成八聚体。观察到活性位点残基的两种不同的保守性模式,这暗示了两种潜在的机制上不同的β-碳酸酐酶。活性位点位于两个单体之间的界面,Cys160,His220和Cys223结合催化锌离子,残基Asp162(由Arg164定向),Gly224,Gln151,Val184,Phe179和Tyr205与底物类似物乙酸相互作用。底物结合基团与α-碳酸酐酶活性位点上的官能团具有一对一的对应关系,相应的残基可被镜面紧密重叠。因此,尽管折叠程度不同,但α-和β-碳酸酐酶已经汇聚在非常相似的活性位点设计上,并且可能具有相同的机理。

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