Mutants of Methylobacterium extorquens and Paracoccus denitrificans deficient in c‐type cytochrome biogenesis synthesise the methylamine‐dehydrogenase polypeptides but cannot assemble the tryptophan‐tryptophylquinone group

Page, M. Dudley; Ferguson, Stuart J.

doi:10.1111/j.1432-1033.1993.tb18425.x

Cited by 30 publications

(25 citation statements)

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“…It has been shown that the TPQ cofactor in CAO (35) and the Cys-Tyr crosslinked cofactor in galactose oxidase (36) are both generated by the copperdependent autocatalytic process of the precursor proteins. On the other hand, the biosynthesis of TTQ in MADH appears to be catalyzed by an enzymatic process, because the absence of one of the genes (mauG) of the 11 genes in the mau operon prevents the maturation of TQQ (37). The biosynthetic process for CTQ in the ␥ subunit of QHNDH may involve an enzyme-mediated process as well.…”

Section: Resultsmentioning

confidence: 99%

Structure of a quinohemoprotein amine dehydrogenase with an uncommon redox cofactor and highly unusual crosslinking

Datta

Mori²,

Takagi³

et al. 2001

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

130

170

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The crystal structure of the heterotrimeric quinohemoprotein amine dehydrogenase from Paracoccus denitrificans has been determined at 2.05-Å resolution. Within an 82-residue subunit is contained an unusual redox cofactor, cysteine tryptophylquinone (CTQ), consisting of an orthoquinone-modified tryptophan side chain covalently linked to a nearby cysteine side chain. The subunit is surrounded on three sides by a 489-residue, four-domain subunit that includes a diheme cytochrome c. Both subunits sit on the surface of a third subunit, a 337-residue seven-bladed ␤-propeller that forms part of the enzyme active site. The small catalytic subunit is internally crosslinked by three highly unusual covalent cysteine to aspartic or glutamic acid thioether linkages in addition to the cofactor crossbridge. The catalytic function of the enzyme as well as the biosynthesis of the unusual catalytic subunit is discussed.

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Section: Resultsmentioning

confidence: 99%

Structure of a quinohemoprotein amine dehydrogenase with an uncommon redox cofactor and highly unusual crosslinking

Datta

Mori²,

Takagi³

et al. 2001

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

130

170

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“…That ccm mutations have pleiotropic effects is becoming increasingly apparent. In the extracellular bacterial systems, ccm has been implicated in manganese oxidation (17,24), gluconate and 2-ketogluconate oxidation (70), methylamine oxidation (64), nicotinic acid hydroxylation (49), copper resistance (86), and the cis-trans isomerization of unsaturated fatty acids (42). Thus, future characterization of our infectivity mutants should provide new insights into ccm and cytochrome c function in particular and bacterial physiology and intracellular infection in general.…”

Section: Discussionmentioning

confidence: 99%

The Cytochrome c Maturation Locus of Legionella pneumophila Promotes Iron Assimilation and Intracellular Infection and Contains a Strain-Specific Insertion Sequence Element

et al. 2002

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Previously, we obtained a Legionella pneumophila mutant, NU208, that is hypersensitive to iron chelators when grown on standard Legionella media. Here, we demonstrate that NU208 is also impaired for growth in media that simply lack their iron supplement. The mutant was not, however, impaired for the production of legiobactin, the only known L. pneumophila siderophore. Importantly, NU208 was also highly defective for intracellular growth in human U937 cell macrophages and Hartmannella and Acanthamoeba amoebae. The growth defect within macrophages was exacerbated by treatment of the host cells with an iron chelator. Sequence analysis demonstrated that the transposon disruption in NU208 lies within an open reading frame that is highly similar to the cytochrome c maturation gene, ccmC. CcmC is generally recognized for its role in the heme export step of cytochrome biogenesis. Indeed, NU208 lacked cytochrome c. Phenotypic analysis of two additional, independently derived ccmC mutants confirmed that the growth defect in low-iron medium and impaired infectivity were associated with the transposon insertion and not an entirely spontaneous second-site mutation. trans-complementation analysis of NU208 confirmed that L. pneumophila ccmC is required for cytochrome c production, growth under low-iron growth conditions, and at least some forms of intracellular infection. Although ccm genes have recently been implicated in iron assimilation, our data indicate, for the first time, that a ccm gene can be required for bacterial growth in an intracellular niche. Complete sequence analysis of the ccm locus from strain 130b identified the genes ccmA-H. Interestingly, however, we also observed that a 1.8-kb insertion sequence element was positioned between ccmB and ccmC. Southern hybridizations indicated that the open reading frame within this element (ISLp 1) was present in multiple copies in some strains of L. pneumophila but was absent from others. These findings represent the first evidence for a transposable element in Legionella and the first identification of an L. pneumophila strain-specific gene.

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“…Examples of an autocatalytic system are the biogenesis of the topaquinone cofactor in copper amine oxidases (15) and of the Cys-Tyr cofactor in galactose oxidase (16), in the latter case with the formation of a thioether linkage. An example of an enzymatic process is the biosynthesis of tryptophan tryptophylquinone in methylamine dehydrogenase, where the absence of one of the genes (mauG) of the 11 genes in the mau operon appears to prevent the maturation of tryptophan tryptophylquinone (17,18).…”

Section: Discrepancy Between Masses Measured By Maldi-tof-ms and Esi-ms-mentioning

confidence: 99%

The Covalent Structure of the Small Subunit fromPseudomonas putida Amine Dehydrogenase Reveals the Presence of Three Novel Types of Internal Cross-linkages, All Involving Cysteine in a Thioether Bond

Vandenberghe¹,

Kim

Devreese³

et al. 2001

Journal of Biological Chemistry

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Pseudomonas putida contains an amine dehydrogenase that is called a quinohemoprotein as it contains a quinone and two hemes c as redox active groups. Amino acid sequence analysis of the smallest (8.5 kDa), quinone-cofactor-bearing subunit of this heterotrimeric enzyme encountered difficulties in the interpretation of the results at several sites of the polypeptide chain. As this suggested posttranslational modifications of the subunit, the structural genes for this enzyme were determined and mass spectrometric de novo sequencing was applied to several peptides obtained by chemical or enzymatic cleavage. In agreement with the interpretation of the X-ray electronic densities in the diffraction data for the holoenzyme, our results show that the polypeptide of the small subunit contains four intrachain cross-linkages in which the sulfur atom of a cysteine residue is involved. Two of these cross-linkages occur with the ␤-carbon atom of an aspartic acid, one with the ␥-carbon atom of a glutamic acid and the fourth with a tryptophanquinone residue, this adduct constituting the enzyme's quinone cofactor, CTQ. The thioether type bond in all four of these adducts has never been found in other proteins. CTQ is a novel cofactor in the series of the recently discovered quinone cofactors.A diversity of enzymes appears to be involved in amine oxidation, as reflected by the number of different cofactors found in the types established so far (1). Based on the natural electron acceptor used, a further distinction can be made between amine oxidases and amine dehydrogenases. Both classes convert amines into their corresponding aldehydes, but oxidases produce toxic peroxides, while the reducing equivalents in the case of dehydrogenases are directly transferred to the respiratory chain (2).Depending on the identity of their cofactor(s), amine dehydrogenases are subdivided into quinoproteins, flavoproteins, quinohemoproteins, and flavohemoproteins (2). Pseudomonas putida strain ATCC 12633, as well as strain IFO 15633, contain a novel type of amine dehydrogenase; a quinohemoprotein (QH-AmDH) 1 as a quinone compound is present in the small subunit and two heme c groups in the large subunit (3). Although the quinone cofactor was not liberated on denaturing the enzyme, spectroscopic data (4) already indicated that it is different from tryptophan tryptophylquinone (5), topaquinone (6), or lysine tyrosylquinone (7), forming part of the protein chain of several amine dehydrogenases (EC 1.4.99.3/4), several amine oxidases (EC 1.4.3.6), and protein-lysine 6-oxidase (EC 1.4.3.13), respectively.To reveal the identity of the quinone cofactor and its position in the protein, the genes for QH-AmDH were cloned and sequenced, and the small subunit subjected to chemical analysis. The latter was carried out in a combination of automated Edman degradation, mass spectrometry, liquid chromatography, and fragmentation MS applied to the underivatized and the derivatized form (the quinone cofactor converted into a hydrazone with a hydrazine) of the small sub...

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Mutants of Methylobacterium extorquens and Paracoccus denitrificans deficient in c‐type cytochrome biogenesis synthesise the methylamine‐dehydrogenase polypeptides but cannot assemble the tryptophan‐tryptophylquinone group

Cited by 30 publications

References 50 publications

Structure of a quinohemoprotein amine dehydrogenase with an uncommon redox cofactor and highly unusual crosslinking

Structure of a quinohemoprotein amine dehydrogenase with an uncommon redox cofactor and highly unusual crosslinking

The Cytochrome c Maturation Locus of Legionella pneumophila Promotes Iron Assimilation and Intracellular Infection and Contains a Strain-Specific Insertion Sequence Element

The Covalent Structure of the Small Subunit fromPseudomonas putida Amine Dehydrogenase Reveals the Presence of Three Novel Types of Internal Cross-linkages, All Involving Cysteine in a Thioether Bond

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