Osuna J, Soberón X, Morett E
Departamento de Reconocimiento Molecular Bioestructura, Universidad Nacional Autónoma de México, México.
Protein Sci. 1997 Mar;6(3):543-55. doi: 10.1002/pro.5560060304.
The expression of genes transcribed by the RNA polymerase with the alternative sigma factor sigma 54 (E sigma 54) is absolutely dependent on activator proteins that bind to enhancer-like sites, located far upstream from the promoter. These unique prokaryotic proteins, known as enhancer-binding proteins (EBP), mediate open promoter complex formation in a reaction dependent on NTP hydrolysis. The best characterized proteins of this family of regulators are NtrC and NifA, which activate genes required for ammonia assimilation and nitrogen fixation, respectively. In a recent IRBM course (@ontiers of protein structure prediction," IRBM, Pomezia, Italy, 1995; see web site http://www.mrc-cpe.cam.uk/irbm-course95/), one of us (J.O.) participated in the elaboration of the proposal that the Central domain of the EBPs might adopt the classical mononucleotide-binding fold. This suggestion was based on the results of a new protein fold recognition algorithm (Map) and in the mapping of correlated mutations calculated for the sequence family on the same mononucleotide-binding fold topology. In this work, we present new data that support the previous conclusion. The results from a number of different secondary structure prediction programs suggest that the Central domain could adopt an alpha/beta topology. The fold recognition programs ProFIT 0.9, 3D PROFILE combined with secondary structure prediction, and 123D suggest a mononucleotide-binding fold topology for the Central domain amino acid sequence. Finally, and most importantly, three of five reported residue alterations that impair the Central domain. ATPase activity of the E sigma 54 activators are mapped to polypeptide regions that might be playing equivalent roles as those involved in nucleotide-binding in the mononucleotide-binding proteins. Furthermore, the known residue substitution that alter the function of the E sigma 54 activators, leaving intact the Central domain ATPase activity, are mapped on region proposed to play an equivalent role as the effector region of the GTPase superfamily.
由RNA聚合酶与替代σ因子σ54(Eσ54)转录的基因表达绝对依赖于激活蛋白,这些激活蛋白与位于启动子上游远处的类增强子位点结合。这些独特的原核生物蛋白,称为增强子结合蛋白(EBP),在依赖于NTP水解的反应中介导开放启动子复合物的形成。该调节因子家族中最具特征的蛋白是NtrC和NifA,它们分别激活氨同化和固氮所需的基因。在最近的一次IRBM课程(“蛋白质结构预测前沿”,IRBM,意大利波梅齐亚,1995年;见网站http://www.mrc-cpe.cam.uk/irbm-course95/)中,我们中的一人(J.O.)参与了关于EBP中央结构域可能采用经典单核苷酸结合折叠的提议的阐述。这个建议基于一种新的蛋白质折叠识别算法(Map)的结果以及针对同一单核苷酸结合折叠拓扑结构计算的序列家族相关突变的映射。在这项工作中,我们展示了支持先前结论的新数据。许多不同二级结构预测程序的结果表明,中央结构域可以采用α/β拓扑结构。折叠识别程序ProFIT 0.9、结合二级结构预测的3D PROFILE和123D表明中央结构域氨基酸序列具有单核苷酸结合折叠拓扑结构。最后,也是最重要的,五个报道的损害中央结构域的残基改变中有三个。Eσ54激活剂的ATPase活性被映射到可能与单核苷酸结合蛋白中参与核苷酸结合的区域发挥等效作用的多肽区域。此外,改变Eσ54激活剂功能但保持中央结构域ATPase活性完整的已知残基替代被映射到提议与GTPase超家族效应器区域发挥等效作用的区域。
