Reinigung und Kristallisation der Thiolase, Untersuchungen zum Wirkungsmechanismus

Gehring, Ulrich; Riepertinger, C.; Lynen, Feodor

doi:10.1111/j.1432-1033.1968.tb00446.x

Cited by 65 publications

(18 citation statements)

References 34 publications

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“…The attractive assumption, early in this work, that the selenium in the thiolase might be in the form of selenocysteine residues proved to be incorrect. Instead, the cysteine residues, as in other thiolases (23,24), presumably are the catalytically active components that undergo acetylation. The cysteine.content of C. kluyveri thiolase (16 per tetramer) determined in this study is similar to the values reported for a thiolase from pig heart (20 per tetramer; 25) and for a thiolase from E. coli (16 per tetramer; 24).…”

Section: Discussionmentioning

confidence: 99%

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Isolation of a selenium-containing thiolase from Clostridium kluyveri: identification of the selenium moiety as selenomethionine.

Hartmanis¹,

Stadtman²

1982

Proc. Natl. Acad. Sci. U.S.A.

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Clostridium kluyveri grown in the presence of 1 ,IM Na2755eO3 produces a thiolase that copurifies with 75Se.Based on several criteria, the selenium moiety in this protein is selenomethionine. The 75Se-labeled amino acid in acid hydrolysates ofthe radioactive protein cochromatographed with authentic selenomethionine on an amino acid analyzer and on TLC plates in acidic and basic solvents. Incubation with S-adenosylmethionine synthetase and ATP converted the 75Se-labeled amino acid to a radioactive basic product that was indistinguishable from authentic Se-adenosylselenomethionine by ion exchange and TLC. The native selenoenzyme, Mr 155,000-158,000, is composed of four subunits of Mr 38,000-40,000. Thiolase of similar molecular weight that is less acidic and lacks selenium is also produced by C. kduyveri. The factors that control the relative levels of the two enzymes in the cell have not been identified.During a survey of various microorganisms for the presence of selenium-modified tRNAs (1), an unknown selenium-containing protein was detected in extracts of the fatty acid-producing anaerobe, Clostridium kluyveri. This protein, labeled with 75Se during growth of the organism in the presence of Na275SeO3, was purified to near homogeneity by a relatively simple procedure prior to its identification as thiolase.t Crude extracts of C. kluyveri proved to contain two proteins of similar molecular weights but different affinities for DEAE-cellulose that exhibited thiolase activity.

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Section: Discussionmentioning

confidence: 99%

“…Only four ofthe cysteine residues (one per subunit) appear to be available in the native protein for reaction with iodoacetamide. Extracts of C. kluyveri are exceptionally rich in thiolase, 17 units/mg of protein (Table 1), as compared with other sources that contain 0.01-0.1 times as much (4,5,23,26).…”

Section: Discussionmentioning

confidence: 99%

Isolation of a selenium-containing thiolase from Clostridium kluyveri: identification of the selenium moiety as selenomethionine.

Hartmanis¹,

Stadtman²

1982

Proc. Natl. Acad. Sci. U.S.A.

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“…Reducing peroxisomal HIBYL-CoA hydrolase activity in chy1 may cause the accumulation of peroxisomal methacrylylCoA, which conjugates to free CoA and proteins containing Cys, thereby disturbing ␤-oxidation either by removing required cofactors or by inactivating required enzymes. One possible target of this inactivation is thiolase, a ␤-oxidation enzyme that has a catalytic, nucleophilic thiol near C-3 of the substrate (49,50). As an Arabidopsis thiolase mutant (ped1) has defects in ␤-oxidation (21) and is IBA-resistant (18), methacrylyl-CoA reaction with the thiolase-active site would likely block the ␤-oxidation of both fatty acids and IBA.…”

Section: Functional Complementation Of Chy1 With a Human Hibyl-mentioning

confidence: 99%

chy1, an Arabidopsis Mutant with Impaired β-Oxidation, Is Defective in a Peroxisomal β-Hydroxyisobutyryl-CoA Hydrolase

Zolman

Monroe-Augustus

Thompson

et al. 2001

Journal of Biological Chemistry

145

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The Arabidopsis chy1 mutant is resistant to indole-3-butyric acid, a naturally occurring form of the plant hormone auxin. Because the mutant also has defects in peroxisomal ␤-oxidation, this resistance presumably results from a reduced conversion of indole-3-butyric acid to indole-3-acetic acid. We have cloned CHY1, which appears to encode a peroxisomal protein 43% identical to a mammalian valine catabolic enzyme that hydrolyzes ␤-hydroxyisobutyryl-CoA. We demonstrated that a human ␤-hydroxyisobutyryl-CoA hydrolase functionally complements chy1 when redirected from the mitochondria to the peroxisomes. We expressed CHY1 as a glutathione S-transferase (GST) fusion protein and demonstrated that purified GST-CHY1 hydrolyzes ␤-hydroxyisobutyryl-CoA. Mutagenesis studies showed that a glutamate that is catalytically essential in homologous enoyl-CoA hydratases was also essential in CHY1. Mutating a residue that is differentially conserved between hydrolases and hydratases established that this position is relevant to the catalytic distinction between the enzyme classes. It is likely that CHY1 acts in peroxisomal valine catabolism and that accumulation of a toxic intermediate, methacrylyl-CoA, causes the altered ␤-oxidation phenotypes of the chy1 mutant. Our results support the hypothesis that the energy-intensive sequence unique to valine catabolism, where an intermediate CoA ester is hydrolyzed and a new CoA ester is formed two steps later, avoids methacrylyl-CoA accumulation.

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“…Thiolase from pig heart is specifically inhibited by iodoacetamide and inhibition of enzyme activity is known to be due to its reaction with a t least three out of a total of 20 residues of cysteine per mole (170000 g) of enzyme protein [1,2]. Moreover when the enzyme-inhibitor compound formed by reaction of the enzyme with i~do- [~~C]acetamide was digested with trypsin three distinct radioactive peptides were found to be present by a combination of ion-exchange chromatography and paper electrophoresis [2a].…”

mentioning

confidence: 99%

The Active Site Cysteines of Thiolase

Harris

Gehring

1970

European Journal of Biochemistry

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Inactivation of thiolase with iodo [l-14C]acetamide has been shown to be due to its reaction with cysteine residues in the enzyme. [ 1 -14C]Carbamoylmethylcysteine was identified as the only product of the reaction and a study of the radioactive peptides that were isolated from a tryptic digest of the [i -14C]carbamoylmethyl-enzyme has shown that the reactive cysteines occur in a unique sequence extending to at least 26 amino acid residues in the primary structure.The enzyme-substrate compound formed when thiolase reacts with [ 1 -14C]acetyl-CoA is shown to contain [14C]acetyl groups bound in thioester linkage to a t least three cysteines per mole. Moreover these residues of [Wlacetyl-cysteine occur exclusively in a sequence that is iden tical to the sequence around the [14C]carbamoylmethylcysteine residues in the enzyme-inhibitor compound, showing that the substrate and the inhibitior react with the same four cysteine residues in the enzyme.These results provide additional evidence for the chemical identity of the four subunits of thiolase.Thiolase from pig heart is specifically inhibited by iodoacetamide and inhibition of enzyme activity is known to be due to its reaction with a t least three out of a total of 20 residues of cysteine per mole (170000 g) of enzyme protein [1,2]. Moreover when the enzyme-inhibitor compound formed by reaction of the enzyme with i~do-[~~C]acetamide was digested with trypsin three distinct radioactive peptides were found to be present by a combination of ion-exchange chromatography and paper electrophoresis [2a]. A t first sight this result could be taken to indicate that the active-site cysteines occur in different sequences in the primary structure of the enzyme. Such a conclusion, however, is not compatible with the results of the peptide mapping studies described in the preceding paper [3]. We have, therefore, reinvestigated the chemical nature of the enzyme-inhibitor compound formed when thiolase is allowed to react with iodo-[14C]acetamide. The three radioactive tryptic peptides have been isolated in pure form and amino acid sequence studies have revealed that they are chemically related and that they form part of a unique sequence around one particular cysteine residue in the primary structure of the enzyme. The reaction of the enzyme with the substrate acetyl-CoA has also been investigated. The acetyl groups that are bound to the enzyme during the enzyme catalysed reaction are shown to be bound in thioester linkage t o cysteine residues, which are moreover the same cysteine residues as were found to react with the inhibitor iodoacetamide.A preliminary account of this work has been published elsewhere [4]. MATERIALS AND METHODS[14C]Acetyl Derivatives Thiolase was prepared from pig heart as previously described 111. The enzyme (35 mg, 0.2 pmoles) was reacted with iodo-[ l-14C]acetamide (2 pmoles, 5.0 mC/mmole) in 0.06 M potassium phosphate pH 7.0 (8.5 ml) at 0". After 30 min 99Oi0 of the original enzyme activity was lost and the reaction was terminated by addition of 3 mmole...

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Reinigung und Kristallisation der Thiolase, Untersuchungen zum Wirkungsmechanismus

Cited by 65 publications

References 34 publications

Isolation of a selenium-containing thiolase from Clostridium kluyveri: identification of the selenium moiety as selenomethionine.

Isolation of a selenium-containing thiolase from Clostridium kluyveri: identification of the selenium moiety as selenomethionine.

chy1, an Arabidopsis Mutant with Impaired β-Oxidation, Is Defective in a Peroxisomal β-Hydroxyisobutyryl-CoA Hydrolase

The Active Site Cysteines of Thiolase

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