Solution Structure of the Actinorhodin Polyketide Synthase Acyl Carrier Protein from Streptomyces coelicolor A3(2) ,

Self Cite

The synthases that produce fatty acids in mammals (FASs) are arranged as large multidomain polypeptides. The growing fatty acid chain is bound covalently during chain elongation and reduction to the acyl carrier protein (ACP) domain that is then able to access each catalytic site. In this work we report the highresolution nuclear magnetic resonance (NMR) solution structure of the isolated rat fatty acid synthase apoACP domain. Fatty acid biosynthesis in mammals is important not only for energy homeostasis and development but also as a potential target for the treatment of obesity (1) and cancer (2). Type I fatty acid synthases (FASs) 3 that catalyze the biosynthesis of fatty acids in mammals, utilize simple acyl units, bound to the phosphopantetheine arm of a holo acyl carrier protein (ACP) domain, for chain initiation and elongation. The recent elucidation of the low resolution structure of the mammalian FAS by x-ray crystallography (3) has provided key structural and mechanistic insights into this important enzyme. Although the resolution of the crystal is insufficient to discern the backbone and side chains, the electron density has permitted the authors to propose a model based on the structures of individual domains and homologous enzymes. The authors have proposed a "head to head" dimeric model that comprises a central core consisting of the enol-reductase, dehydratase (DH), and ketosynthase with the malonyl transferase and ketoreductase domains being located peripherally. Dimerization occurs through association of the KS domains. Notable absences in the crystal structure are the locations of the peripheral ACP and thioesterase domains, suggesting that the positions of the ACP and thioesterase domains are relatively mobile compared with the core of the FAS. In comparison, bacterial Type II FASs consist of discrete monofunctional proteins (4). Structural studies of the Type II FAS ACP components are particularly well developed and have revealed the structural basis of acyl chain binding and the phenomenon of conformational switching. The crystal structures of Escherichia coli FAS butyryl (5), hexanoyl-, heptanoyl-, and decanoyl-ACPs (6) and nuclear magnetic resonance (NMR) structures of spinach FAS decanoyl-and stearoyl-ACPs have been reported (7). These structures reveal that during fatty acid biosynthesis, fully saturated acyl chains are sequestered within a central cavity in the ACP formed through conformational changes in the protein. The fatty acid chain is sequestered within the hydrophobic core of the ACP perhaps to protect the thioester moiety from hydrolysis. Binding of the acyl chain also influences the dynamics of the ACPs. Spinach FAS holo-ACP exists in equilibrium between a folded and largely disordered form, however, upon acylation this equilibrium is shifted toward the folded form. At present the physiological role of switching of this, and other ACPs, is unknown (8, 9). It has been suggested that switching confers allosteric regulation of the ACP, whereby its interaction with other enzymes...

Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 95%

A Mammalian Type I Fatty Acid Synthase Acyl Carrier Protein Domain Does Not Sequester Acyl Chains

Płoskoń¹,

Arthur

Evans

et al. 2008

Self Cite

“…It is unclear whether this inhibition reflects interactions between the apoACP protein and MAT or KS/CLF or both. Since the solution structures of several Type II ACPs have been solved (31)(32)(33)(34)(35)(36)(37)(38), further studies into the structural basis for these molecular recognition properties could provide fundamentally new insights into the importance of protein-protein interactions in regulating Type II PKS function and specificity.…”

Section: Discussionmentioning

confidence: 99%

Kinetic Analysis of the Actinorhodin Aromatic Polyketide Synthase

Dreier¹,

Shah²,

Khosla³

1999

Type II polyketide synthases (PKSs) are bacterial multienzyme systems that catalyze the biosynthesis of a broad range of natural products. A core set of subunits, consisting of a ketosynthase, a chain length factor, an acyl carrier protein (ACP) and possibly a malonyl CoA: ACP transacylase (MAT) forms a "minimal" PKS. They generate a poly-␤-ketone backbone of a specified length from malonyl-CoA derived building blocks. Here we (a) report on the kinetic properties of the actinorhodin minimal PKS, and (b) present further data in support of the requirement of the MAT. Kinetic analysis showed that the apoACP is a competitive inhibitor of minimal PKS activity, demonstrating the importance of proteinprotein interactions between the polypeptide moiety of the ACP and the remainder of the minimal PKS. In further support of the requirement of MAT for PKS activity, two new findings are presented. First, we observe hyperbolic dependence of PKS activity on MAT concentration, saturating at very low amounts (half-maximal rate at 19.7 ؎ 5.1 nM). Since MAT can support PKS activity at less than 1/100 the typical concentration of the ACP and ketosynthase/chain length factor components, it is difficult to rule out the presence of trace quantities of MAT in a PKS reaction mixture. Second, an S97A mutant was constructed at the nucleophilic active site of the MAT. Not only can this mutant protein support PKS activity, it is also covalently labeled by [ 14 C]malonyl-CoA, demonstrating that the serine nucleophile (which has been the target of PMSF inhibition in earlier studies) is dispensible for MAT activity in a Type II PKS system.

“…To study the ACP binding ability of FabG and FabG mutants, 1 M biotinylated ACP was incubated with different concentrations (30 nM to 2 M) of Histagged FabG at room temperature in a 384-well ProxiPlate (Packard Instrument Co.). After a 30-min incubation, streptavidin donor beads and nickel chelate acceptor beads (50 g/ml final concentration for each bead, (His) 6 Tag detection system, Packard Instrument Co.) were added to the above solutions. The reaction mixtures were then incubated for 1 h before being read by Fusion TM Universal Microplate Analyzer (Packard Instrument Co.), with excitation at 680 nm and emission at 600 nm.…”

Section: Materials-amershammentioning

confidence: 99%

Key Residues Responsible for Acyl Carrier Protein and β-Ketoacyl-Acyl Carrier Protein Reductase (FabG) Interaction

Zhang¹,

Zheng

et al. 2003

133

148

We tested this hypothesis by mutating two surface residues, Arg-129 and Arg-172, located in a hydrophobic patch adjacent to the active site entrance on ␤-ketoacyl-ACP reductase (FabG). Enzymatic analysis showed that the mutant enzymes were compromised in their ability to utilize ACP thioester substrates but were fully active in assays with a substrate analog. Direct binding assays and competitive inhibition experiments showed that the FabG mutant proteins had reduced affinities for ACP. Chemical shift perturbation protein NMR experiments showed that FabG-ACP interactions occurred along the length of ACP helix ␣2 and extended into the adjacent loop-2 region to involve Ile-54. These data confirm a role for the highly conserved electronegative/hydrophobic residues along ACP helix ␣2 in recognizing a constellation of Arg residues embedded in a hydrophobic patch on the surface of its partner enzymes, and reveal a role for the loop-2 region in the conformational change associated with ACP binding. The specific FabG-ACP interactions involve the most conserved ACP residues, which accounts for the ability of ACPs and the type II proteins from different species to function interchangeably.Fatty acid biosynthesis in bacteria and plants is carried out by a series of enzymes that are collectively known as the type II fatty-acid synthase and is most extensively studied in the Escherichia coli system (1, 2). ACP 1 is a small, acidic protein that functions as the central acyl group carrier in type II fatty-acid synthase systems. The ACPs are rod-shaped proteins with a preponderance of acidic residues organized into four ␣-helices (3-7). The acyl intermediates are attached to the terminal sulfhydryl of the 4Ј-phosphopantetheine prosthetic group (8), which is attached via a phosphodiester linkage to Ser-36 located at the beginning of the second helical segment. The primary gene product is an apoprotein that is converted to ACP by the transfer of the 4Ј-phosphopantetheine moiety of CoA to Ser-36 by [ACP]synthase (AcpS) (9, 10). ACP performs two functions. First, it sequesters the growing acyl chain from the aqueous environment, and second, upon binding to one of the type II proteins, it releases its grip on the fatty acid, which is inserted into the active site cavity of the enzyme. ACPs are widely distributed in nature and are easily recognized by their significant primary sequence identity, particularly at the prosthetic group attachment site and extending along helix ␣2 (11). These similarities are thought to underlie the observation that ACPs from virtually any source are substrates for AcpS and function with the fatty acid biosynthetic enzymes of E. coli (11). However, the individual enzymes of type II fatty acid synthesis do not share a primary structure motif that would define the presence of a common ACP-binding motif.The molecular details that govern the specific interactions between ACP and the type II enzymes are poorly known. The analysis of the binding of ACP to FabH points to ionic interactions playing a determinant ...