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GTP-dependent activation of urease apoprotein in complex with the UreD UreF and UreG accessory proteins

机译:与UreDUreF和UreG辅助蛋白复合的脲酶脱辅基蛋白的GTP依赖性激活

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摘要

Syntheses of metal-containing enzymes often require the participation of accessory proteins. The roles played by many of these accessory proteins are poorly characterized. Klebsiella aerogenes urease, a nickel-containing enzyme, provides an ideal system to study metallocenter assembly. Here, we describe a method for isolating a complex containing urease apoprotein and the UreD, UreF, and UreG accessory proteins. We demonstrate that urease apoprotein in this complex is activated to near wild-type enzyme levels when incubated with nickel ions and high (≈100 mM) concentrations of bicarbonate. Significantly, we also observed nickel-dependent activation at physiologically relevant (≈100 μM) bicarbonate levels, but only in the presence of GTP. Based on studies involving a nonhydrolyzable analog of GTP, we conclude that nucleotide hydrolysis, not just binding, is required for this process. The critical nucleotide-binding site was localized to UreG on the basis of experiments using a variant complex. These studies highlight the relevance of the UreD-UreF-UreG-urease apoprotein complex to nickel metallocenter assembly and explain the previously identified in vivo energy requirement for urease activation.
机译:含金属酶的合成通常需要辅助蛋白的参与。许多这些辅助蛋白所起的作用还很差。产气克雷伯菌尿素酶(一种含镍酶)为研究金属中心组装提供了理想的系统。在这里,我们描述了一种分离包含尿素酶载脂蛋白和UreD,UreF和UreG辅助蛋白的复合物的方法。我们证明,当与镍离子和高浓度(约100 mM)的碳酸氢盐一起孵育时,该复合物中的脲酶载脂蛋白被激活至接近野生型酶水平。重要的是,我们还观察到在生理相关的碳酸氢根水平(约100μM)下镍依赖性活化,但仅在GTP存在的情况下。基于涉及GTP不可水解类似物的研究,我们得出结论,此过程需要核苷酸水解,而不仅仅是结合。在使用变体复合物的实验的基础上,关键核苷酸结合位点定位于UreG。这些研究突出了UreD-UreF-UreG-脲酶脱辅基蛋白复合物与镍金属中心组装体的相关性,并解释了先前确定的尿素酶激活体内能量需求。

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