Pyruvate formate-lyase (inactive form) and pyruvate formate-lyase activating enzyme of Escherichia coli: Isolation and structural properties |
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Authors: | Harald Conradt Marita Hohmann-Berger Hans-Peter Hohmann Hans P. Blaschkowski Joachim Knappe |
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Affiliation: | Institut für Biologische Chemie, Universität Heidelberg, Im Neuenheimer Feld 501, D-69 Heidelberg, Federal Republic of Germany |
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Abstract: | The catalytically active form (Ea) of pyruvate formate-lyase in Escherichia coli cells is generated from an inactive form of the enzyme (Ei) through a post-translational process that requires a distinct activating enzyme and is linked to the cleavage of adenosylmethionine to methionine and 5′-deoxyadenosine. Ei and the activating enzyme were purified to homogeneity and structurally characterized. Ei has an α2 oligomeric structure (2 × 85 kDa) and contains no cofactor. The amino acid composition has been determined. Out of a total of six cysteinyl residues per subunit, one shows an unusually fast reaction with iodoacetate (k2 = 7 (m? s?) at pH 6.8, 30 °C), which is accompanied by loss of the activatability of the enzyme. The 1500-fold purified activating enzyme is a monomeric protein of 30 kDa. It contains a covalently bound, as yet unidentified chromophoric factor which has an optical absorption peak at 388 nm. Further studies of the in situ state of pyruvate formate-lyase detected a reversible backconversion of the active form Ea into Ei when anaerobic cells become nutrient-depleted. |
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Keywords: | To whom all correspondence should be sent. |
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