首页> 美国卫生研究院文献>Acta Crystallographica Section F: Structural Biology and Crystallization Communications >The crystallization of apo-form UMP kinase from Xanthomonas campestris is significantly improved in a strong magnetic field
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The crystallization of apo-form UMP kinase from Xanthomonas campestris is significantly improved in a strong magnetic field

机译:在强磁场中来自油菜黄单胞菌的脱辅基形式UMP激酶的结晶得到显着改善

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摘要

Bacterial UMP kinases (UMPKs) are crucial enzymes that are responsible for microbial UTP biosynthesis. Interestingly, eukaryotic and prokaryotic cells use different enzymes for UMP-phosphorylation reactions. Prokaryotic UMPKs are thus believed to be potential targets for antimicrobial drug development. Here, the cloning, expression and crystallization of SeMet-substituted XC1936, a bacterial UMPK from Xanthomonas campestris pathovar campestris, are reported. The crystallization of the apo-form UMPK was found to be significantly improved in a strong magnetic field; the crystals diffracted to a resolution of 2.35 Å, a dramatic improvement over the original value of 3.6 Å. Preliminary structural analyses of apo-form XC1936 using crystals grown in a strong magnetic field clearly reveal well defined loop regions involved in substrate-analogue binding that were previously not visible. Crystallization in a strong magnetic field thus was found to be indispensable in determining the flexible region of the XC1936 UMPK structure.
机译:细菌UMP激酶(UMPKs)是负责微生物UTP生物合成的关键酶。有趣的是,真核和原核细胞使用不同的酶进行UMP磷酸化反应。因此,原核UMPK被认为是抗菌药物开发的潜在靶标。在这里,报道了SeMet-取代的XC1936(一种来自喜多单胞菌(Xanthomonas campestris)的病原体campestris)的UMPK的克隆,表达和结晶。发现在强磁场中,脱辅基形式的UMPK的结晶得到明显改善。晶体衍射到2.35Å的分辨率,比3.6Å的原始值有了显着提高。使用在强磁场中生长的晶体对脱辅基形式XC1936进行的初步结构分析清楚地揭示了以前不可见的参与底物-类似物结合的明确定义的环区域。因此,在确定XC1936 UMPK结构的柔性区域时,发现在强磁场中结晶是必不可少的。

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