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Building reactive copper centers in human carbonic anhydrase II

机译:在人类碳酸酐酶II中建立活性铜中心

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摘要

Reengineering metalloproteins to generate new biologically relevant metal centers is an effective a way to test our understanding of the structural and mechanistic features that steer chemical transformations in biological systems. Here, we report thermodynamic data characterizing the formation of two type-2 copper sites in carbonic anhydrase and experimental evidence showing one of these new, copper centers has characteristics similar to a variety of well-characterized copper centers in synthetic models and enzymatic systems. Human carbonic anhydrase II is known to bind two Cu~(2+) ions; these binding events were explored using modern isothermal titration calorimetry techniques that have become a proven method to accurately measure metal-binding thermodynamic parameters. The two Cu~(2+)-binding events have different affinities (K a approximately 5 × 10~(12) and 1 × 10~(10)), and both are enthalpically driven processes. Reconstituting these Cu~(2+) sites under a range of conditions has allowed us to assign the Cu~(2+)-binding event to the three-histidine, native, metal-binding site. Our initial efforts to characterize these Cu~(2+) sites have yielded data that show distinctive (and noncoupled) EPR signals associated with each copper-binding site and that this reconstituted enzyme can activate hydrogen peroxide to catalyze the oxidation of 2-aminophenol.
机译:重新设计金属蛋白以生成新的生物学上相关的金属中心是一种有效的方法,可以检验我们对引导生物系统中化学转化的结构和机制特征的理解。在这里,我们报告了表征碳酸酐酶中两个2型铜位点形成的热力学数据,并且实验证据表明这些新的铜中心之一具有与合成模型和酶系统中各种特征鲜明的铜中心相似的特征。已知人类碳酸酐酶II结合两个Cu〜(2+)离子;这些结合事件是使用现代等温滴定量热技术进行的,这些技术已成为一种准确测量金属结合热力学参数的可靠方法。两个Cu〜(2+)结合事件具有不同的亲和力(K a约为5×10〜(12)和1×10〜(10)),并且都是受焓驱动的过程。在一定条件下重构这些Cu〜(2+)位点使我们能够将Cu〜(2+)结合事件分配给三个组氨酸的天然金属结合位点。我们为表征这些Cu〜(2+)位点所做的初步努力已获得数据,这些数据显示了与每个铜结合位点相关的独特(和非耦合)EPR信号,并且这种重组酶可以激活过氧化氢以催化2-氨基苯酚的氧化。

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