Trapping the dynamic acyl carrier protein in fatty acid biosynthesis

A highly specific chemical crosslinking method is used to trap a complex between an acyl carrier protein and a fatty acid dehydratase during fatty acid biosynthesis; subsequent X-ray crystallography, NMR spectroscopy and molecular dynamics simulations techniques enable the detailed study of this com...

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Veröffentlicht in:Nature (London) Jg. 505; H. 7483; S. 427 - 431
Hauptverfasser: Nguyen, Chi, Haushalter, Robert W., Lee, D. John, Markwick, Phineus R. L., Bruegger, Joel, Caldara-Festin, Grace, Finzel, Kara, Jackson, David R., Ishikawa, Fumihiro, O’Dowd, Bing, McCammon, J. Andrew, Opella, Stanley J., Tsai, Shiou-Chuan, Burkart, Michael D.
Format: Journal Article
Sprache:Englisch
Veröffentlicht: London Nature Publishing Group UK 16.01.2014
Nature Publishing Group
Schlagworte:
631/535/1266
631/92/287/1183
631/92/60
Acyl Carrier Protein - chemistry
Acyl Carrier Protein - metabolism
Binding Sites
Biosynthesis
Catalytic Domain
Cross-Linking Reagents - chemistry
Crosslinked polymers
Crystal structure
Crystallography, X-Ray
Dehydration
E coli
Enzymes
Escherichia coli - chemistry
Fatty Acid Synthase, Type II - chemistry
Fatty Acid Synthase, Type II - metabolism
Fatty acids
Fatty Acids - biosynthesis
Histidine - metabolism
Humanities and Social Sciences
Hydro-Lyases - chemistry
Hydro-Lyases - metabolism
Infectious diseases
letter
Magnetic Resonance Spectroscopy
Metabolites
Models, Molecular
Molecular Dynamics Simulation
multidisciplinary
NMR
Nuclear magnetic resonance
Physiological aspects
Protein Binding
Protein Interaction Maps
Proteins
Science
Synthesis
United States
ISSN:0028-0836, 1476-4687, 1476-4687
Online-Zugang:Volltext
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Zusammenfassung:A highly specific chemical crosslinking method is used to trap a complex between an acyl carrier protein and a fatty acid dehydratase during fatty acid biosynthesis; subsequent X-ray crystallography, NMR spectroscopy and molecular dynamics simulations techniques enable the detailed study of this complex. Acyl carrier protein structures revealed During fatty acid and polyketide biosynthesis the growing polymer chain is stabilized by acyl carrier proteins (ACPs), but the transient nature of the process makes it difficult to visualize the molecular mechanisms involved. Two papers published in this issue of Nature use strategies that circumvent this problem. Ali Masoudi et al . solve the X-ray crystal structures of an ACP from Escherichia coli bound to LpxD, an acyltransferase in the lipid A biosynthetic pathway, in three different states: an intact acyl-ACP, a hydrolysed-acyl-ACP, and a holo-ACP form. Alignment of these structures makes it possible to visualize the conformational changes that take place in the ACP during catalysis. Chi Nguyen et al . use a crosslinking probe to tether an ACP to an active site histidine of one of its catalytic enzymes, the dehydratase FabA from E. coli . They obtain a high-resolution X-ray crystal structure of the stabilized ACP–FabA complex and use NMR spectroscopy to probe the dynamics of ACP–FabA interactions. Their experiments support a 'switchblade' model. This crosslink-probe approach can be applied to other carrier protein partners in metabolic and signalling pathways. Acyl carrier protein (ACP) transports the growing fatty acid chain between enzymatic domains of fatty acid synthase (FAS) during biosynthesis 1 . Because FAS enzymes operate on ACP-bound acyl groups, ACP must stabilize and transport the growing lipid chain 2 . ACPs have a central role in transporting starting materials and intermediates throughout the fatty acid biosynthetic pathway 3 , 4 , 5 . The transient nature of ACP–enzyme interactions impose major obstacles to obtaining high-resolution structural information about fatty acid biosynthesis, and a new strategy is required to study protein–protein interactions effectively. Here we describe the application of a mechanism-based probe that allows active site-selective covalent crosslinking of AcpP to FabA, the Escherichia coli ACP and fatty acid 3-hydroxyacyl-ACP dehydratase, respectively. We report the 1.9 Å crystal structure of the crosslinked AcpP–FabA complex as a homodimer in which AcpP exhibits two different conformations, representing probable snapshots of ACP in action: the 4′-phosphopantetheine group of AcpP first binds an arginine-rich groove of FabA, then an AcpP helical conformational change locks AcpP and FabA in place. Residues at the interface of AcpP and FabA are identified and validated by solution nuclear magnetic resonance techniques, including chemical shift perturbations and residual dipolar coupling measurements. These not only support our interpretation of the crystal structures but also provide an animated view of ACP in action during fatty acid dehydration. These techniques, in combination with molecular dynamics simulations, show for the first time that FabA extrudes the sequestered acyl chain from the ACP binding pocket before dehydration by repositioning helix III. Extensive sequence conservation among carrier proteins suggests that the mechanistic insights gleaned from our studies may be broadly applicable to fatty acid, polyketide and non-ribosomal biosynthesis. Here the foundation is laid for defining the dynamic action of carrier-protein activity in primary and secondary metabolism, providing insight into pathways that can have major roles in the treatment of cancer, obesity and infectious disease.
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These authors contributed equally to this work.
ISSN:0028-0836
1476-4687
1476-4687
DOI:10.1038/nature12810