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钴(II)碳酸酐酶的电子顺磁共振研究。低自旋氰化物配合物。

Electron-paramagnetic-resonance studies on cobalt(II) carbonic anhydrase. Low-spin cyanide complexes.

作者信息

Cockle S A

出版信息

Biochem J. 1974 Mar;137(3):587-96. doi: 10.1042/bj1370587.

Abstract

The low-spin cyanide complexes of three Co(II) carbonic anhydrases were investigated by electron paramagnetic resonance (e.p.r.) at 9 and 35GHz. Well-defined and closely axial spectra were obtained only in the absence of oxygen. Several mole equivalents of cyanide were required for complete formation of the complexes in frozen solution, although large excesses caused abstraction of the cobalt. Experiments with [(13)C]cyanide showed that the low-spin complexes contained two CN(-) groups in an environment similar to that of the in-plane ligands in Co(CN)(5). A combined e.p.r. and spectrophotometric titration confirmed the presence of two CN(-) ligands. A 5-co-ordinate square pyramidal structure involving three protein ligands was proposed. The dicyanide complex could be oxygenated reversibly, producing a characteristic new e.p.r. spectrum. The O(2) molecule was thought to occupy the remaining octahedral metal site in a formally Co(III) species. The optical spectrum of the dicyanide lacked the prominent d-d bands of the high-spin monocyanide. Both e.p.r. and optical data indicated that the low-spin complex was formed much more fully in frozen solution than at room temperature. Differences in behaviour between the high- and low-activity enzymes suggested some variation in conformational flexibility at the metal binding site.

摘要

利用电子顺磁共振(e.p.r.)在9GHz和35GHz频率下对三种钴(II)碳酸酐酶的低自旋氰化物配合物进行了研究。仅在无氧条件下才能获得明确且近似轴向的光谱。在冷冻溶液中,完全形成配合物需要几摩尔当量的氰化物,不过过量过多会导致钴被提取。用[(13)C]氰化物进行的实验表明,低自旋配合物含有两个氰基(CN-),其所处环境与[Co(CN)5](3-)中面内配体的环境相似。电子顺磁共振和分光光度滴定相结合证实了两个氰基(CN-)配体的存在。有人提出了一种涉及三个蛋白质配体的五配位正方锥结构。二氰化物配合物可被可逆地氧化,产生特征性的新电子顺磁共振光谱。氧分子被认为占据了形式上为钴(III)物种中剩余的八面体金属位点。二氰化物的光谱缺乏高自旋单氰化物中显著的d-d带。电子顺磁共振和光谱数据均表明,低自旋配合物在冷冻溶液中比在室温下形成得更完全。高活性和低活性酶之间行为的差异表明金属结合位点的构象灵活性存在一些变化。

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METAL-BINDING PROPERTIES OF HUMAN ERYTHROCYTE CARBONIC ANHYDRASES.人红细胞碳酸酐酶的金属结合特性
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