Structural insights into the synthesis of FMN in prokaryotic organisms.

B. Herguedas, Isaias Lans, María Sebastián, J. Hermoso, M. Martínez-Júlvez, M. Medina
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引用次数: 23

Abstract

Riboflavin kinases (RFKs) catalyse the phosphorylation of riboflavin to produce FMN. In most bacteria this activity is catalysed by the C-terminal module of a bifunctional enzyme, FAD synthetase (FADS), which also catalyses the transformation of FMN into FAD through its N-terminal FMN adenylyltransferase (FMNAT) module. The RFK module of FADS is a homologue of eukaryotic monofunctional RFKs, while the FMNAT module lacks homologyto eukaryotic enzymes involved in FAD production. Previously, the crystal structure of Corynebacterium ammoniagenes FADS (CaFADS) was determined in its apo form. This structure predicted a dimer-of-trimers organization with the catalytic sites of two modules of neighbouring protomers approaching each other, leading to a hypothesis about the possibility of FMN channelling in the oligomeric protein. Here, two crystal structures of the individually expressed RFK module of CaFADS in complex with the products of the reaction, FMN and ADP, are presented. Structures are complemented with computational simulations, binding studies and kinetic characterization. Binding of ligands triggers dramatic structural changes in the RFK module, which affect large portions of the protein. Substrate inhibition and molecular-dynamics simulations allowed the conformational changes that take place along the RFK catalytic cycle to be established. The influence of these conformational changes in the FMNAT module is also discussed in the context of the full-length CaFADS protomer and the quaternary organization.
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原核生物中FMN合成的结构见解。
核黄素激酶(RFKs)催化核黄素磷酸化产生FMN。在大多数细菌中,这种活性是由双功能酶FAD合成酶(FADS)的c端模块催化的,FADS也通过其n端FMN腺苷基转移酶(FMNAT)模块催化FMN转化为FAD。FADS的RFK模块是真核单功能RFKs的同源物,而FMNAT模块与参与FAD产生的真核酶缺乏同源性。此前,氨根棒状杆菌FADS (CaFADS)的晶体结构以载脂蛋白形式进行了测定。该结构预测了三聚体的二聚体组织,相邻原聚体的两个模块的催化位点相互靠近,从而导致了关于低聚蛋白中FMN通道可能性的假设。本文给出了单独表达的CaFADS RFK模块与反应产物FMN和ADP配合物的两种晶体结构。结构辅以计算模拟,结合研究和动力学表征。配体的结合会引发RFK模块的剧烈结构变化,从而影响蛋白质的大部分。底物抑制和分子动力学模拟使得沿着RFK催化循环发生的构象变化得以建立。这些构象变化对FMNAT模块的影响也在全长CaFADS原聚体和四级组织的背景下进行了讨论。
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来源期刊
自引率
13.60%
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审稿时长
3 months
期刊介绍: Acta Crystallographica Section D welcomes the submission of articles covering any aspect of structural biology, with a particular emphasis on the structures of biological macromolecules or the methods used to determine them. Reports on new structures of biological importance may address the smallest macromolecules to the largest complex molecular machines. These structures may have been determined using any structural biology technique including crystallography, NMR, cryoEM and/or other techniques. The key criterion is that such articles must present significant new insights into biological, chemical or medical sciences. The inclusion of complementary data that support the conclusions drawn from the structural studies (such as binding studies, mass spectrometry, enzyme assays, or analysis of mutants or other modified forms of biological macromolecule) is encouraged. Methods articles may include new approaches to any aspect of biological structure determination or structure analysis but will only be accepted where they focus on new methods that are demonstrated to be of general applicability and importance to structural biology. Articles describing particularly difficult problems in structural biology are also welcomed, if the analysis would provide useful insights to others facing similar problems.
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