Institute of Biophysics and Physical Biochemistry, Regensburg Center for Biochemistry, University of Regensburg, Regensburg, Germany.
Appl Environ Microbiol. 2024 May 21;90(5):e0057224. doi: 10.1128/aem.00572-24. Epub 2024 May 3.
Multi-resistant bacteria are a rapidly emerging threat to modern medicine. It is thus essential to identify and validate novel antibacterial targets that promise high robustness against resistance-mediating mutations. This can be achieved by simultaneously targeting several conserved function-determining protein-protein interactions in enzyme complexes from prokaryotic primary metabolism. Here, we selected two evolutionary related glutamine amidotransferase complexes, aminodeoxychorismate synthase and anthranilate synthase, that are required for the biosynthesis of folate and tryptophan in most prokaryotic organisms. Both enzymes rely on the interplay of a glutaminase and a synthase subunit that is conferred by a highly conserved subunit interface. Consequently, inhibiting subunit association in both enzymes by one competing bispecific inhibitor has the potential to suppress bacterial proliferation. We comprehensively verified two conserved interface hot-spot residues as potential inhibitor-binding sites by demonstrating their crucial role in subunit association and enzymatic activity. For target validation, we generated genomically modified strains in which subunit association was disrupted by modifying these central interface residues. The growth of such strains was drastically retarded on liquid and solid minimal medium due to a lack of folate and tryptophan. Remarkably, the bacteriostatic effect was observed even in the presence of heat-inactivated human plasma, demonstrating that accessible host metabolite concentrations do not compensate for the lack of folate and tryptophan within the tested bacterial cells. We conclude that a potential inhibitor targeting both enzyme complexes will be effective against a broad spectrum of pathogens and offer increased resilience against antibiotic resistance.
Antibiotics are indispensable for the treatment of bacterial infections in human and veterinary medicine and are thus a major pillar of modern medicine. However, the exposure of bacteria to antibiotics generates an unintentional selective pressure on bacterial assemblies that over time promotes the development or acquisition of resistance mechanisms, allowing pathogens to escape the treatment. In that manner, humanity is in an ever-lasting race with pathogens to come up with new treatment options before resistances emerge. In general, antibiotics with novel modes of action require more complex pathogen adaptations as compared to chemical derivates of existing entities, thus delaying the emergence of resistance. In this contribution, we use modified strains to validate two novel targets required for folate and tryptophan biosynthesis that can potentially be targeted by one and the same bispecific protein-protein interaction inhibitor and promise increased robustness against bacterial resistances.
多耐药菌是现代医学面临的一个迅速出现的威胁。因此,识别和验证新的抗菌靶标至关重要,这些靶标承诺对耐药性介导的突变具有高度的稳健性。这可以通过同时针对原核初级代谢物中酶复合物的几个保守功能决定的蛋白-蛋白相互作用来实现。在这里,我们选择了两种进化相关的谷氨酰胺酰胺转移酶复合物,即氨基脱氧胆色素合酶和邻氨基苯甲酸合酶,它们是大多数原核生物中叶酸和色氨酸生物合成所必需的。这两种酶都依赖于谷氨酰胺酶和一个由高度保守的亚基界面赋予的合成酶亚基的相互作用。因此,一种竞争的双特异性抑制剂抑制两种酶中亚基的结合有可能抑制细菌的增殖。我们通过证明这些保守的界面热点残基在亚基结合和酶活性中的关键作用,全面验证了两个保守的界面热点残基作为潜在的抑制剂结合位点。为了进行靶标验证,我们通过修饰这些核心界面残基,在基因组上修饰了 菌株,从而破坏了亚基的结合。由于缺乏叶酸和色氨酸,这些菌株在液体和固体最小培养基中的生长受到严重阻碍。值得注意的是,即使在热灭活的人血浆存在的情况下,也观察到抑菌作用,这表明可利用的宿主代谢物浓度不能补偿测试细菌细胞内叶酸和色氨酸的缺乏。我们的结论是,针对两种酶复合物的潜在抑制剂将对广谱病原体有效,并提供对抗生素耐药性的更高抵抗力。
抗生素在人类和兽医医学中对细菌感染的治疗是不可或缺的,因此是现代医学的主要支柱。然而,细菌暴露于抗生素会对细菌组装产生无意的选择性压力,随着时间的推移,这会促进耐药机制的发展或获得,使病原体能够逃避治疗。通过这种方式,人类与病原体进行着一场永无止境的竞赛,以在出现耐药性之前找到新的治疗方案。一般来说,与现有实体的化学衍生物相比,具有新型作用模式的抗生素需要更复杂的病原体适应,从而延迟耐药性的出现。在本研究中,我们使用修饰的 菌株来验证两种新型靶标,这些靶标是叶酸和色氨酸生物合成所必需的,它们可能可以被一种双特异性的蛋白-蛋白相互作用抑制剂靶向,并对细菌的耐药性具有更高的稳健性。
