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ENZYMES AND PROTEINS

Purification and Characterization of Active-Site Components of the Putative p-Cresol Methylhydroxylase Membrane Complex from Geobacter metallireducens

Jörg Johannes, Alexander Bluschke, Nico Jehmlich, Martin von Bergen, Matthias Boll
Jörg Johannes
1Institute of Biochemistry, University of Leipzig, Brüderstraβe 34, 04103 Leipzig, Germany
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Alexander Bluschke
1Institute of Biochemistry, University of Leipzig, Brüderstraβe 34, 04103 Leipzig, Germany
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Nico Jehmlich
2Department for Proteomics, Helmholtz Center for Environmental Research, Permoserstraβe 15, 04318 Leipzig, Germany
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Martin von Bergen
2Department for Proteomics, Helmholtz Center for Environmental Research, Permoserstraβe 15, 04318 Leipzig, Germany
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Matthias Boll
1Institute of Biochemistry, University of Leipzig, Brüderstraβe 34, 04103 Leipzig, Germany
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  • For correspondence: boll@uni-leipzig.de
DOI: 10.1128/JB.00790-08
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ABSTRACT

p-Cresol methylhydroxylases (PCMH) from aerobic and facultatively anaerobic bacteria are soluble, periplasmic flavocytochromes that catalyze the first step in biological p-cresol degradation, the hydroxylation of the substrate with water. Recent results suggested that p-cresol degradation in the strictly anaerobic Geobacter metallireducens involves a tightly membrane-bound PCMH complex. In this work, the soluble components of this complex were purified and characterized. The data obtained suggest a molecular mass of 124 ± 15 kDa and a unique αα′β2 subunit composition, with α and α′ representing isoforms of the flavin adenine dinucleotide (FAD)-containing subunit and β representing a c-type cytochrome. Fluorescence and mass spectrometric analysis suggested that one FAD was covalently linked to Tyr394 of the α subunit. In contrast, the α′ subunit did not contain any FAD cofactor and is therefore considered to be catalytically inactive. The UV/visible spectrum was typical for a flavocytochrome with two heme c cofactors and one FAD cofactor. p-Cresol reduced the FAD but only one of the two heme cofactors. PCMH catalyzed both the hydroxylation of p-cresol to p-hydroxybenzyl alcohol and the subsequent oxidation of the latter to p-hydroxybenzaldehyde in the presence of artificial electron acceptors. The very low Km values (1.7 and 2.7 μM, respectively) suggest that the in vivo function of PCMH is to oxidize both p-cresol and p-hydroxybenzyl alcohol. The latter was a mixed inhibitor of p-cresol oxidation, with inhibition constants of a K ic (competitive inhibition) value of 18 ± 9 μM and a K iu (uncompetitive inhibition) value of 235 ± 20 μM. A putative functional model for an unusual PCMH enzyme is presented.

  • Copyright © 2008 American Society for Microbiology
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Purification and Characterization of Active-Site Components of the Putative p-Cresol Methylhydroxylase Membrane Complex from Geobacter metallireducens
Jörg Johannes, Alexander Bluschke, Nico Jehmlich, Martin von Bergen, Matthias Boll
Journal of Bacteriology Sep 2008, 190 (19) 6493-6500; DOI: 10.1128/JB.00790-08

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Purification and Characterization of Active-Site Components of the Putative p-Cresol Methylhydroxylase Membrane Complex from Geobacter metallireducens
Jörg Johannes, Alexander Bluschke, Nico Jehmlich, Martin von Bergen, Matthias Boll
Journal of Bacteriology Sep 2008, 190 (19) 6493-6500; DOI: 10.1128/JB.00790-08
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KEYWORDS

Bacterial Proteins
Geobacter
membrane proteins
Mixed Function Oxygenases

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