Structure, mechanism and regulation of pyruvate carboxylase

PC (pyruvate carboxylase) is a biotin-containing enzyme that catalyses the HCO3−- and MgATP-dependent carboxylation of pyruvate to form oxaloacetate. This is a very important anaplerotic reaction, replenishing oxaloacetate withdrawn from the tricarboxylic acid cycle for various pivotal biochemical pathways. PC is therefore considered as an enzyme that is crucial for intermediary metabolism, controlling fuel partitioning toward gluconeogenesis or lipogenesis and in insulin secretion. The enzyme was discovered in 1959 and over the last decade there has been much progress in understanding its structure and function. PC from most organisms is a tetrameric protein that is allosterically regulated by acetyl-CoA and aspartate. High-resolution crystal structures of the holoenzyme with various ligands bound have recently been determined, and have revealed details of the binding sites and the relative positions of the biotin carboxylase, carboxyltransferase and biotin carboxyl carrier domains, and also a unique allosteric effector domain. In the presence of the allosteric effector, acetyl-CoA, the biotin moiety transfers the carboxy group between the biotin carboxylase domain active site on one polypeptide chain and the carboxyltransferase active site on the adjacent antiparallel polypeptide chain. In addition, the bona fide role of PC in the non-gluconeogenic tissues has been studied using a combination of classical biochemistry and genetic approaches. The first cloning of the promoter of the PC gene in mammals and subsequent transcriptional studies reveal some key cognate transcription factors regulating tissue-specific expression. The present review summarizes these advances and also offers some prospects in terms of future directions for the study of this important enzyme.

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Pyruvate carboxylase catalysis of phosphate transfer between carbamoyl phosphate and ADP

Biochemical Journal ◽

10.1042/bj2730443 ◽

1991 ◽

Vol 273 (2) ◽

pp. 443-448 ◽

Cited By ~ 13

Author(s):

P V Attwood ◽

B D L A Graneri

Keyword(s):

Active Site ◽

Pyruvate Carboxylase ◽

Reverse Reaction ◽

Carbamoyl Phosphate ◽

Acetyl Coa ◽

Essential Requirement ◽

Pyruvate Carboxylation ◽

Ionizable Residues ◽

Ph Profiles

In a reaction that is analogous to the phosphorylation of ADP from carboxyphosphate, pyruvate carboxylase catalyses the formation of ATP from carbamoyl phosphate and ADP at a rate that is about 0.3% of the pyruvate-carboxylation reaction and about 3% of the full reverse reaction. Acetyl-CoA stimulates the phosphorylation of ADP from carbamoyl phosphate but is not an essential requirement of the reaction. Mg2+ also stimulates the reaction, and in the range of Mg2+ concentrations considered the effect of V is much larger in the absence of acetyl-CoA than in its presence. Acetyl-CoA and Mg2+ may be acting in a co-operative way to stimulate the phosphorylation of ADP in a similar way to their effects on the pyruvate-carboxylation reaction. The phosphorylation of ADP by carbamoyl phosphate is also stimulated by the presence of biotin in the part of the active site where this reaction occurs, but again it is not absolutely required for the reaction to proceed. The pH profiles of the phosphorylation of ADP by carbamoyl phosphate indicate that there are at least two ionizable residues involved in the reaction, one of which probably has a role in the release of carbamate from the active site.

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Bicarbonate-dependent ATP cleavage catalysed by pyruvate carboxylase in the absence of pyruvate

Biochemical Journal ◽

10.1042/bj2871011 ◽

1992 ◽

Vol 287 (3) ◽

pp. 1011-1017 ◽

Cited By ~ 20

Author(s):

P V Attwood ◽

B D L A Graneri

Keyword(s):

Reaction Mechanism ◽

Atpase Activity ◽

Active Site ◽

Pyruvate Carboxylase ◽

Substrate Inhibition ◽

Cleavage Reaction ◽

Acetyl Coa ◽

Enzyme Preparations ◽

Pyruvate Carboxylation ◽

Rate Of Movement

Preparations of pyruvate carboxylase catalyse the cleavage of MgATP in the absence of pyruvate and acetyl-CoA. The rate of this cleavage is higher in the presence of HCO3- than in its absence. Incubation of the enzyme preparations with an excess of the pyruvate carboxylase inhibitor, avidin, completely abolishes the pyruvate carboxylating activity of the enzyme preparations but only abolishes the HCO3(-)-dependent MgATP cleaving activity, with no effect on the HCO3(-)-independent ATPase activity. The HCO3(-)-dependent MgATP cleavage is also sensitive to inhibition by a pyruvate carboxylase inhibitor, oxamate, and the dependence of the reaction on the free Mg2+ concentration is similar to that of the pyruvate-carboxylation reaction, whereas the HCO3(-)-independent MgATP cleavage is not dependent on the concentration of free Mg2+ in the range tested. This indicates that MgATP cleavage by pyruvate carboxylase is entirely dependent on the presence of HCO3- and that there may be a low level of ATPase contamination in the enzyme preparations. In addition, inhibition of the HCO3(-)-dependent MgATP cleavage by both avidin and oxamate indicate that although biotin does not directly participate in the reaction, its presence is required in that part of the active site of the enzyme. The rate of HCO3(-)-dependent MgATP cleavage is about 0.07% of that of the full pyruvate carboxylation reaction under similar conditions with saturating substrates. The reaction mechanism is sequential with respect to MgATP and HCO3- addition and Mg2+ adds at equilibrium before MgATP. Acetyl-CoA stimulates the HCO3(-)-dependent MgATP cleavage at low MgATP concentrations, with the stimulation being greater at low Mg2+ concentrations. At high levels of MgATP in the presence of acetyl-CoA, substrate inhibition is evident and is more pronounced at increasing concentrations of Mg2+. This inhibition appears to be, at least in part, caused by inhibition of decarboxylation of the enzyme-carboxybiotin complex by the binding to this complex of Mg2+ and MgATP, which probably act to reduce the rate of movement of carboxybiotin from the site of the MgATP cleavage reaction to that of the pyruvate carboxylation reaction where it is unstable and decarboxylates.

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Factors that influence the translocation of the N-carboxybiotin moiety between the two sub-sites of pyruvate carboxylase

Biochemical Journal ◽

10.1042/bj1990603 ◽

1981 ◽

Vol 199 (3) ◽

pp. 603-609 ◽

Cited By ~ 31

Author(s):

G J Goodall ◽

G S Baldwin ◽

J C Wallace ◽

D B Keech

Keyword(s):

Dissociation Constant ◽

Carboxy Group ◽

Active Site ◽

Pyruvate Carboxylase ◽

Alternative Substrate ◽

Acetyl Coa ◽

Low Concentrations ◽

Acid Substrate ◽

Allosteric Activator ◽

Rate Of Movement

The active site of pyruvate carboxylase, like those of all biotin-dependent carboxylases, is believed to consist of two spatially distinct sub-sites with biotin acting as a mobile carboxy-group carrier oscillating between the two sub-sites. Some of the factors that influence the location and rate of movement of the N-carboxybiotin were studied. The rate of carboxylation of the alternative substrate, 2-oxobutyrate, was measured at 0 degrees C in an assay system where the isolated enzyme--[14C]carboxybiotin was the carboxy-group donor. The results are consistent with the hypothesis that the location of the carboxybiotin in the active site is determined by the presence of Mg2+, acetyl-CoA and the oxo acid substrate. The presence of Mg2+ favours the holding of the complex at the first sub-site, whereas alpha-oxo acids induce the complex to move to the second sub-site. At low concentrations pyruvate induces this movement but does not efficiently act as a carboxy-group acceptor; hydroxypyruvate, glyoxylate and oxamate, though not carboxylated, still induce the movement. The allosteric activator acetyl-CoA exerts only a slight stimulation on the rate of translocation to the second sub-site, and this stimulation arises from an increase in the dissociation constant for Mg2+.

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Inhibition of CO2 fixation in group D streptococci

Canadian Journal of Microbiology ◽

10.1139/m69-009 ◽

1969 ◽

Vol 15 (1) ◽

pp. 57-60 ◽

Cited By ~ 8

Author(s):

Victor F. Lachica ◽

Paul A. Hartman

Keyword(s):

Phosphoenolpyruvate Carboxylase ◽

Pyruvate Carboxylase ◽

Co2 Fixation ◽

Tricarboxylic Acid Cycle ◽

Inhibitory Effect ◽

Tricarboxylic Acid ◽

Acetyl Coa ◽

Acid Cycle ◽

Tricarboxylic Acid Cycle Intermediates ◽

Group D

The stimulatory effect of acetyl-CoA and the inhibitory effect by L-aspartate and some intermediates of the tricarboxylic acid cycle in the assimilation of CO2 by crude extracts of group D streptococci suggest that the pyruvate carboxylase of Streptococcus faecium and the phosphoenolpyruvate carboxylase of S. bovis are allosteric enzymes. This implies that these enzymes are sites for the control of the amount of aspartate and of the tricarboxylic acid cycle intermediates synthesized.

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Ligand-induced conformational transitions and secondary-structure composition of chicken liver pyruvate carboxylase

Biochemical Journal ◽

10.1042/bj1770697 ◽

1979 ◽

Vol 177 (2) ◽

pp. 697-705 ◽

Cited By ~ 8

Author(s):

Karen S. McGurk ◽

H. Olin Spivey

Keyword(s):

Secondary Structure ◽

Pyruvate Carboxylase ◽

Conformational Transitions ◽

Sulphonic Acid ◽

Chicken Liver ◽

Stopped Flow ◽

Acetyl Coa ◽

Allosteric Effector ◽

Fluorescence Measurements ◽

Secondary Structure Composition

Apparent conformational transitions induced in chicken liver pyruvate carboxylase by substrates, KHCO3 and MgATP, and the allosteric effector, acetyl-CoA, were studied by using the fluorescent probe, 8-anilinonaphthalene-1-sulphonic acid and c.d. Fluorescence measurements were made with both conventional and stopped-flow spectrophotometers. Additions of acetyl-CoA and/or ATP to the enzyme-probe solutions quenched fluorescence of the probe by the following cumulative amounts regardless of the sequence of additions: acetyl-CoA, 10–13%; ATP, 21–24%; acetyl-CoA plus ATP, about 35%. Additions of KHCO3 had no effect on the fluorescence. The rates of quenching by acetyl-CoA and MgATP (in the presence of acetyl-CoA) were too rapid to measure by stopped-flow kinetic methods, but kinetics of the MgATP effect (in the absence of acetyl-CoA) indicate three unimolecular transitions after the association step. The negligible effect of the probe on enzyme catalytic activity, a preservation of the near-u.v. c.d. effect of MgATP and acetyl-CoA in the presence of the probe and no observable unimolecular transitions after binding of the probe to the enzyme indicate that the probe had no deleterious effect on the enzyme. In contrast with results with 8-anilinonaphthalene-1-sulphonic acid, fluorescence of the ε-derivative of acetyl-CoA or ATP [fluorescent analogues; Secrist, Barrio, Leonard & Weber (1972) Biochemistry11, 3499–3506] was not changed when either one was added to the enzyme. Secondary-structure composition of chicken liver pyruvate carboxylase estimated from the far-u.v. c.d. spectrum of the enzyme is 27% helix, 7% β-pleated sheet and 66% other structural types.

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Allosteric regulation of the biotin-dependent enzyme pyruvate carboxylase by acetyl-CoA

Biochemical Society Transactions ◽

10.1042/bst20120041 ◽

2012 ◽

Vol 40 (3) ◽

pp. 567-572 ◽

Cited By ~ 24

Author(s):

Abdussalam Adina-Zada ◽

Tonya N. Zeczycki ◽

Martin St. Maurice ◽

Sarawut Jitrapakdee ◽

W. Wallace Cleland ◽

...

Keyword(s):

Active Site ◽

Pyruvate Carboxylase ◽

Structural Effects ◽

Reaction Conditions ◽

Acetyl Coa ◽

X Ray ◽

Allosteric Interactions ◽

Crystallographic Structures ◽

And Staphylococcus Aureus ◽

Allosteric Activator

The activity of the biotin-dependent enzyme pyruvate carboxylase from many organisms is highly regulated by the allosteric activator acetyl-CoA. A number of X-ray crystallographic structures of the native pyruvate carboxylase tetramer are now available for the enzyme from Rhizobium etli and Staphylococcus aureus. Although all of these structures show that intersubunit catalysis occurs, in the case of the R. etli enzyme, only two of the four subunits have the allosteric activator bound to them and are optimally configured for catalysis of the overall reaction. However, it is apparent that acetyl-CoA binding does not induce the observed asymmetrical tetramer conformation and it is likely that, under normal reaction conditions, all of the subunits have acetyl-CoA bound to them. Thus the activation of the enzyme by acetyl-CoA involves more subtle structural effects, one of which may be to facilitate the correct positioning of Arg353 and biotin in the biotin carboxylase domain active site, thereby promoting biotin carboxylation and, at the same time, preventing abortive decarboxylation of carboxybiotin. It is also apparent from the crystal structures that there are allosteric interactions induced by acetyl-CoA binding in the pair of subunits not optimally configured for catalysis of the overall reaction.

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The atypical velocity response by pyruvate carboxylase to increasing concentrations of acetyl-coenzyme A

Biochemical Journal ◽

10.1042/bj1790497 ◽

1979 ◽

Vol 179 (3) ◽

pp. 497-502 ◽

Cited By ~ 6

Author(s):

Simon B. Easterbrook-Smith ◽

Anne J. Campbell ◽

D. Bruce Keech ◽

John C. Wallace

Keyword(s):

Velocity Profile ◽

Pyruvate Carboxylase ◽

Degree Of Saturation ◽

Acetyl Coa ◽

Reaction Velocity ◽

Low Protein ◽

Allosteric Effector ◽

Velocity Response ◽

Hill Coefficients ◽

Hydrolysis Of

An investigation was made of the interaction of pyruvate carboxylase with its allosteric effector, acetyl-CoA, and the velocity profile of the deacylation of acetyl-CoA as a function of acetyl-CoA concentration indicated that this ligand does not bind to this enzyme in a positive homotropic co-operative manner. An examination was therefore made of the factors that contribute to the sigmoidicity of the rate curves obtained for pyruvate carboxylation with various concentrations of acetyl-CoA. Hill coefficients for acetyl-CoA obtained with both sheep and chicken liver pyruvate carboxylases were found to be dependent on the fixed pyruvate concentration used in the assay solution. Thus, by varying the acetyl-CoA concentration, the degree of saturation of the enzyme by pyruvate was also changed. A further consequence of non-saturating concentrations of pyruvate was that the non-productive hydrolysis of the enzyme– carboxybiotin complex increased, resulting in an under-estimate of the reaction velocity measured by oxaloacetate formation. Another factor contributing to the sigmoidicity is that, at non-saturating concentrations of acetyl-CoA, the enzyme undergoes inactivation upon dilution to low protein concentrations, again resulting in an under-estimate of the reaction velocity. Under conditions where none of the above factors was operating and the only effect of varying acetyl-CoA concentrations was to alter the proportion of the enzyme catalysing the carboxylation reaction at acetyl-CoA-dependent and -independent rates, the sigmoidicity of the acetyl-CoA velocity profile was completely eliminated.

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Synthesis of pyruvate carboxylase from its apoenzyme and (+)-biotin in Bacillus stearothermophilus. Mechanism and control of the reaction

Biochemical Journal ◽

10.1042/bj1220663 ◽

1971 ◽

Vol 122 (5) ◽

pp. 663-669 ◽

Cited By ~ 9

Author(s):

T. K. Sundaram ◽

J. J. Cazzulo ◽

H. L. Kornberg

Keyword(s):

Pyruvate Carboxylase ◽

Thermal Denaturation ◽

Bacillus Stearothermophilus ◽

The Other ◽

Acetyl Coa ◽

Allosteric Effector ◽

Allosteric Effectors ◽

Hill Coefficients ◽

And Control ◽

The Hill

1. Acetyl-CoA acts as a positive allosteric effector in the formation of active pyruvate carboxylase from its apoenzyme, ATP and (+)-biotin which is catalysed by holoenzyme synthetase; this effect is counteracted by l-aspartate. 2. The Hill coefficients (apparent n values) were approximately 2 for acetyl-CoA and 4 for l-aspartate; the n value for each effector remained constant when the concentration of the other effector was varied. 3. Active pyruvate carboxylase was formed also when the apoenzyme was incubated with holoenzyme synthetase and synthetic biotinyl-5′-AMP; acetyl-CoA and l-aspartate affected this process as they did the overall reaction from (+)-biotin and ATP. 4. When hydroxylamine replaced the apoenzyme, holoenzyme synthetase catalysed the formation of biotinylhydroxamate from (+)-biotin and ATP. This reaction was not affected by the allosteric effectors. 5. The apoenzyme was protected against thermal denaturation by acetyl-CoA and, to a lesser degree, by l-aspartate. The holoenzyme synthetase was not markedly protected by these effectors. 6. It is concluded that the allosteric effectors act on the apoenzyme and not the synthetase.

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Dinuclear nickel complexes modeling the structure and function of the acetyl CoA synthase active site

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.0900433106 ◽

2009 ◽

Vol 106 (29) ◽

pp. 11862-11866 ◽

Cited By ~ 32

Author(s):

M. Ito ◽

M. Kotera ◽

T. Matsumoto ◽

K. Tatsumi

Keyword(s):

Active Site ◽

Nickel Complexes ◽

Structure And Function ◽

Acetyl Coa ◽

And Function

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Fe(2)OG: an integrated HMM profile-based web server to predict and analyze putative non-haem iron(II)- and 2-oxoglutarate-dependent dioxygenase function in protein sequences

BMC Research Notes ◽

10.1186/s13104-021-05477-z ◽

2021 ◽

Vol 14 (1) ◽

Author(s):

Siddhartha Kundu

Keyword(s):

Amino Acid ◽

Water Molecule ◽

Active Site ◽

Ferrous Iron ◽

Web Server ◽

Protein Sequences ◽

Diverse Group ◽

And Function ◽

Functionally Diverse ◽

Haem Iron

Abstract Objective Non-haem iron(II)- and 2-oxoglutarate-dependent dioxygenases (i2OGdd), are a taxonomically and functionally diverse group of enzymes. The active site comprises ferrous iron in a hexa-coordinated distorted octahedron with the apoenzyme, 2-oxoglutarate and a displaceable water molecule. Current information on novel i2OGdd members is sparse and relies on computationally-derived annotation schema. The dissimilar amino acid composition and variable active site geometry thereof, results in differing reaction chemistries amongst i2OGdd members. An additional need of researchers is a curated list of sequences with putative i2OGdd function which can be probed further for empirical data. Results This work reports the implementation of $$Fe\left(2\right)OG$$ F e 2 O G , a web server with dual functionality and an extension of previous work on i2OGdd enzymes $$\left(Fe\left(2\right)OG\equiv \{H2OGpred,DB2OG\}\right)$$ F e 2 O G ≡ { H 2 O G p r e d , D B 2 O G } . $$Fe\left(2\right)OG$$ F e 2 O G , in this form is completely revised, updated (URL, scripts, repository) and will strengthen the knowledge base of investigators on i2OGdd biochemistry and function. $$Fe\left(2\right)OG$$ F e 2 O G , utilizes the superior predictive propensity of HMM-profiles of laboratory validated i2OGdd members to predict probable active site geometries in user-defined protein sequences. $$Fe\left(2\right)OG$$ F e 2 O G , also provides researchers with a pre-compiled list of analyzed and searchable i2OGdd-like sequences, many of which may be clinically relevant. $$Fe(2)OG$$ F e ( 2 ) O G , is freely available (http://204.152.217.16/Fe2OG.html) and supersedes all previous versions, i.e., H2OGpred, DB2OG.

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