Gerichtete Evolution als Methode zur Erzeugung enantioselektiver Cyclohexanonmonooxygenasen (CHMOs) für die Katalyse von Baeyer-Villiger-Reaktionen

Schneider, Toni.

January 2005

Bochum, Univ., Diss., 2005. / Computerdatei im Fernzugriff.

Cyclohexanon-Monooxygenase

Gerichtete Evolution als Methode zur Erzeugung enantioselektiver Cyclohexanonmonooxygenasen (CHMOs) für die Katalyse von Baeyer-Villiger-Reaktionen

Schneider, Toni.

January 2005

Bochum, Universiẗat, Diss., 2005.

Cyclohexanon-Monooxygenase

Dinuclear Schiff base complexes as models for metallobiosites

Ryan, Sara Jane

January 1998

No description available.

572

Dioxygen carrier; Monooxygenase

Studies on metabolic sulphoxidation of alkyl and aryl thioethers : Role of cytochrome P-450 and FAD-containing monooxygenases

Houdi, A. A.

January 1986

No description available.

615.1

Drug monooxygenase inhibition

The production of cytochrome P-450 by Saccharomyces cerevisiae during computer-controlled batch fermentations

Dorr, Arthur

January 1991

No description available.

572

Monooxygenase enzymes

Tyrosinase nanocapsules for the lowering of systemic tyrosine levels for the treatment of melanoma

Fustier, Caroline.

January 1900

Thesis (M.Eng.). / Written for the Dept. of Biomedical Engineering. Title from title page of PDF (viewed 2008/01/14). Includes bibliographical references.

Elucidating the flavin reductase mechanism in the alkanesulfonate monooxygenase system from Escherichia coli

Gao, Benlian, Ellis, Holly R.

January 2006

Dissertation (Ph.D.)--Auburn University,2006. / Abstract. Vita. Includes bibliographic references (p.139-152).

Structural dynamics and ligand binding in kynurenine-3-monooxygenase

Wilkinson, Martin

January 2013

Kynurenine 3-monooxygenase is a FAD-dependent aromatic hydroxylase (FAH) which is a widely suggested therapeutic target for controlling the balance of bioactive metabolite levels produced by the mammalian kynurenine pathway (KP). Prior to starting this work no structural information was known for the enzyme, with studies of the human form complicated by the presence of a C-terminal transmembrane helix. The bacterial Pseudomonas fluorescens enzyme (PfKMO) lacks the transmembrane region and has been previously characterised by Crozier-Reabe and Moran [1, 2]. Therefore PfKMO, which shares 32 % sequence identity with the human enzyme, was selected as a target for structure solution. Initial substrate bound PfKMO crystals showed poor X-ray diffraction. Subsequent growth optimisation and the generation of a C252S/C461S PfKMO mutant (dm2) yielded crystals suitable for structure solution. Selenomethioninelabelled substrate bound dm2 crystals were used to solve the first structure to a resolution of 3.40 Å. With just one protein molecule per asymmetric unit, a high solvent content was responsible for the poor diffraction properties of this crystal form. The overall fold resembled that of other FAH enzymes with a Rossmann-fold based FADbinding domain above a buried substrate binding pocket. Interestingly PfKMO possesses an additional, novel C-terminal domain that caps the back of the substrate-binding pocket on the opposite side to the flavin. Residues proposed to be involved in substrate binding were identified and shown to be highly conserved among mammalian KMO sequences. Subsequently single crystals of substrate-free dm2 PfKMO were obtained and showed significantly stronger diffraction due to new lattice packing in an orthorhombic space group bearing four molecules per asymmetric unit. The structure was solved to a resolution of 2.26 Å and revealed a clear conformational change of the novel C-terminal domain. This movement opens a potential route of substrate/product exchange between bulk solvent and the active site. The investigation of a set of C-terminal mutants further explored the relevance and mechanics of the conformational change. In addition the presence of chloride ions in the substrate-free crystal growth solution caused a small number of localised subtle alterations to the structure, with a potential chloride binding site identified adjacent to the flavin cofactor. This may have relevance for the observed inhibition of PfKMO activity by monovalent anions – a feature widely common to FAH enzymes [3]. The first discovered KMO inhibitors were analogues of the substrate L-Kyn, however one such compound (m-NBA) was recently shown to instigate uncoupled NADPH oxidation leading to the release of cytotoxic hydrogen peroxide [1]. A set of substrate analogues were tested and characterised for inhibition of PfKMO. The picture was shown to be complex as some substrate analogues completely inhibited the enzyme whilst the binding of some still stimulated low-levels of NADPH oxidation. Crystallographic studies with m-NBA and 3,4-dichlorobenzoylalanine (3,4-CBA) bound revealed indistinguishable structures from that of substrate-bound PfKMO. These studies suggest that the analogue 3,4CBA is a potent PfKMO inhibitor whose therapeutic potential may be re-visited. The previous most potent KMO inhibitor whose structure was not analogous to the substrate was Ro 61-8048 [4], which unfortunately did not pass pre-clinical safety tests. A novel series of 1,2,4-oxadiazole amides based on the structure of Ro 61-8048 was created by Gavin Milne (PhD, University of St Andrews) and tested on PfKMO. Rounds of refinement led to the discovery and refinement of low nanomolar competitive inhibitors of the bacterial enzyme. PfKMO was co-crystallised with each of the four most potent compounds forming a third different lattice arrangement, which yielded structures to resolutions of 2.15-2.40 Å. The structures displayed conformational changes resembling the substrate-free fold possibly caused by displacement of a crucial substrate-binding residue, R84. Overall the wealth of structural data obtained may be transferable to predictions about the structural features of human KMO and to the rational design of therapeutic inhibitors. The potent novel inhibitors tested may additionally present a new exciting development for the therapeutic inhibition of human KMO.

Functional roles of conserved active site amino acids in the desulfonation reaction catalyzed by the alkanesulfonate monooxygenase from Escheria coli

Carpenter, Russell, Ellis, Holly R.,

January 2008

Thesis (Ph. D.)--Auburn University. / Abstract. Vita. Includes bibliographical references (p. 156-168).

Catalytic mechanism of a flavin-dependent alkanesulfonate monoxygenase from Escherichia coli

Zhan, Xuanzhi, Ellis, Holly R.,

January 2008

Thesis (Ph. D.)--Auburn University, 2008. / Abstract. Vita. Includes bibliographical references (p. 154-166).