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Structure and function of FusB: an elongation factor G-binding fusidic acid resistance protein active in ribosomal translocation and recycling

机译:FusB的结构和功能:一种在核糖体转运和回收中具有活性的延伸因子G结合夫西地酸抗性蛋白

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Fusidic acid (FA) is a bacteriostatic antibiotic that locks elongation factor G (EF-G) to the ribosome after GTP hydrolysis during elongation and ribosome recycling. The plasmid pUB101-encoded protein FusB causes FA resistance in clinical isolates of Staphylococcus aureus through an interaction with EF-G. Here, we report 1.6 and 2.3 ? crystal structures of FusB. We show that FusB is a two-domain protein lacking homology to known structures, where the N-terminal domain is a four-helix bundle and the C-terminal domain has an alpha/beta fold containing a C4 treble clef zinc finger motif and two loop regions with conserved basic residues. Using hybrid constructs between S. aureus EF-G that binds to FusB and Escherichia coli EF-G that does not, we show that the sequence determinants for FusB recognition reside in domain IV and involve the C-terminal helix of S. aureus EF-G. Further, using kinetic assays in a reconstituted translation system, we demonstrate that FusB can rescue FA inhibition of tRNA translocation as well as ribosome recycling. We propose that FusB rescues S. aureus from FA inhibition by preventing formation or facilitating dissociation of the FA-locked EF-G–ribosome complex.
机译:夫西地酸(FA)是一种抑菌抗生素,在伸长和核糖体回收过程中GTP水解后,将伸长因子G(EF-G)锁定在核糖体上。质粒pUB101编码的蛋白FusB通过与EF-G相互作用在金黄色葡萄球菌临床分离株中引起FA抗性。在这里,我们报告1.6和2.3? FusB的晶体结构。我们显示FusB是一个缺乏已知结构同源性的两个域蛋白,其中N端结构域是一个四螺旋束,C端结构域具有一个包含C4高音谱号锌指基序和两个的α/β折叠带有保守碱性残基的环区域。使用与FusB结合的金黄色葡萄球菌EF-G和不与FusB结合的大肠杆菌EF-G之间的杂交构建体,我们显示FusB识别的序列决定子位于域IV中,并涉及金黄色葡萄球菌EF-C的C末端螺旋。 G。此外,在重组翻译系统中使用动力学测定,我们证明FusB可以挽救FA对tRNA转运以及核糖体回收的抑制作用。我们建议FusB通过阻止FA锁定的EF-G-核糖体复合物的形成或促进其解离,从FA抑制中拯救金黄色葡萄球菌。

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