Rates of the Phthalate Dioxygenase Reaction with Oxygen Are Dramatically Increased by Interactions with Phthalate and Phthalate Oxygenase Reductase

Tarasev, Michael; Rhames, Frank; Ballou, David P.

doi:10.1021/bi0490587

Cited by 29 publications

(54 citation statements)

References 29 publications

(67 reference statements)

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“…Plasmids containing WT PDO and D178N and D178A variants genes were constructed and the proteins were expressed and purified as described previously (14). Concentrations of enzymes were determined spectrophotometrically using Δε 575 = 2.38 mM −1 cm −1 and Δε 466 = 17.54 mM −1 cm −1 for the extinction coefficient differences between oxidized and reduced PDO and PDR, respectively.…”

Section: Methodsmentioning

confidence: 99%

“…Concentrations of enzymes were determined spectrophotometrically using Δε 575 = 2.38 mM −1 cm −1 and Δε 466 = 17.54 mM −1 cm −1 for the extinction coefficient differences between oxidized and reduced PDO and PDR, respectively. PDO activity was determined in steady-state assays as described previously (14). When necessary, Fe(NH 4 ) 2 (SO 4 ) 2 (FAS), prepared as an anaerobic solution of known concentration, was added.…”

Section: Methodsmentioning

confidence: 99%

“…When necessary, Fe(NH 4 ) 2 (SO 4 ) 2 (FAS), prepared as an anaerobic solution of known concentration, was added. PDO-APO, which lacks iron in the mononuclear center, and a less stringent preparation (PDO-APO 20 ), which contained about 2.2 Fe/monomer, were prepared as described previously (14). Iron content in PDO was determined by Inductively Coupled Plasma High Resolution Mass Spectrometry (ICP) using a Finnegan Element Instrument from Thermo Finnegan Co.…”

Section: Methodsmentioning

confidence: 99%

“…Similar to NDO (9) and BZDO (28), when the Rieske center in PDO is reduced, NO binds to the mononuclear iron only when substrate is present (14). However, when the Rieske center is oxidized, NO can bind both in the presence and in the absence of the substrate (14). Such gating of NO (and by extension, possibly O 2 ) binding by the redox state of the Rieske center and the availability of the substrate appears to be a common feature of this family of Rieske dioxygenases.…”

Section: Epr Spectra Of Pdo-no Complexesmentioning

confidence: 99%

“…Certain caveats should be noted concerning the exact geometry of binding in the non-heme enzymes; for example, while the binding of oxygen in NDO was shown to be side-on to the mononuclear iron (12), the binding to NO was shown to occur in an end-on fashion (13). Using NO as a limited model for oxygen binding at the Fe(II) of the mononuclear center , it was found that NO can bind to the mononuclear Fe(II) if the Rieske center is oxidized, but not when it is reduced, unless substrate is also bound at the mononuclear center (9,14). Thus, there is important communication between the Rieske and mononuclear sites, and this communication has been proposed to be due to His-104, His-213, and Asp-205 in NDO (9).…”

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confidence: 99%

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The “Bridging” Aspartate 178 in Phthalate Dioxygenase Facilitates Interactions between the Rieske Center and the Iron(II)−Mononuclear Center

et al. 2006

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Phthalate dioxygenase (PDO) and its reductase are parts of a two-component Rieske dioxygenase system that initiates the aerobic breakdown of phthalate by forming cis-4,5-dihydro-4,5-dihydroxyphthalate (DHD). Aspartate D178 in PDO, located near its ferrous mononuclear center, is highly conserved among Rieske dioxygenases. The analogous aspartate has been implicated in electron transfer between the mononuclear iron and Rieske center in naphthalene dioxygenase (Parales, R.E. et. al. (1999) J Bacteriol 181, 1831-1837 and in substrate binding and oxygen reactivity in anthranilate dioxygenase (Beharry, Z.M. et. al (2003), Biochemistry 42, 13625-13636). The effects of substituting D178 in PDO with alanine or asparagine on the reactivity of the Rieske centers, phthalate hydroxylation, and coupling of Rieske center oxidation to DHD formation were studied previously (Pinto, A., Tarasev, M., and Ballou, D. P. (2006) Biochemistry in press). This work describes effects that D178N and D178A substitutions have on the interactions between the Rieske and mononuclear centers in PDO. The mutations affected protonation of the Rieske center histidine and conformation of subunits within the PDO multimer to create a more open structure with more solvent-accessible Rieske centers. When the Rieske centers in PDO were oxidized, D178N and D178A substitutions disrupted communication between the Rieske and Fe-mononuclear centers. This was shown by the lack of perturbations of the UV-vis spectra on phthalate binding to the D178N and D178A variants, as opposed to that observed in WT PDO. However, when the Rieske center was in the reduced state, communication between the centers was not disrupted. Phthalate binding similarly affected the rates of oxidation of the reduced Rieske center in both WT and mutant PDO. Nitric Oxide binding at the Fe(II) mononuclear center, as detected by EPR spectrometry of the Fe(II) nitrosyl complex, was regulated by the redox state of the Rieske center. When the Rieske center was oxidized in either WT or D178N PDO, NO bound to the mononuclear iron in the presence or absence of phthalate. However, when the Rieske center was reduced, NO bound only when phthalate was present. These findings are discussed in terms of the "communication functions" performed by the bridging Asp-178.Phthalate dioxygenase (PDO) and its reductase are parts of a two-component enzyme system (PDS) in Burkholderia cepacia DB01 that initiates the aerobic breakdown of phthalate by forming cis-4,5-dihydro-4,5-dihydroxyphthalate (DHD). PDS comprises the monomeric phthalate dioxygenase reductase (PDR), an enzyme that contains both FMN and a plant-type [2Fe-2S] ferredoxin, and a Rieske dioxygenase (PDO), an α 6 multimer that contains Rieske and ferrous mononuclear centers. Mononuclear iron and Rieske centers on each subunit in Rieske oxygenases are shown to be separated by more than 40 Å (2), making direct electron *To whom correspondence should be addressed. Email: dballou@umich.edu NIH Public Access transfer unfavorable (3). However, as s...

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Epr Spectra Of Pdo-no Complexesmentioning

confidence: 99%

mentioning

confidence: 99%

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The “Bridging” Aspartate 178 in Phthalate Dioxygenase Facilitates Interactions between the Rieske Center and the Iron(II)−Mononuclear Center

et al. 2006

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Cytochrome P450 Redox Partner Systems: Biodiversity and Biotechnological Implications

Munro

Girvan

McVey

et al. 2007

Modern Biooxidation

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Oxygen activation by mononuclear nonheme iron dioxygenases involved in the degradation of aromatics

Wang

Liu

2017

J Biol Inorg Chem

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Molecular oxygen is utilized in numerous metabolic pathways fundamental for life. Mononuclear nonheme iron-dependent oxygenase enzymes are well-known for their involvement in some of these pathways, activating O2 so that oxygen atoms can be incorporated into their primary substrates. These reactions often initiate pathways that allow organisms to use stable organic molecules as sources of carbon and energy for growth. From the myriad of reactions in which these enzymes are involved, this perspective recounts the general mechanisms of aromatic dihydroxylation and oxidative ring cleavage, both of which are ubiquitous chemical reactions found in life-sustaining processes. The organic substrate provides all four electrons required for oxygen activation and insertion in the reactions mediated by extradiol and intradiol ring-cleaving catechol dioxygenases. In contrast, two of the electrons are provided by NADH in the cis-dihydroxylation mechanism of Rieske dioxygenases. The catalytic nonheme Fe center, with the aid of active site residues, facilitates these electron transfers to O2 as key elements of the activation processes. This review discusses some general questions for the catalytic strategies of oxygen activation and insertion into aromatic compounds employed by mononuclear nonheme iron-dependent dioxygenases. These include: (1) how oxygen is activated, (2) whether there are common intermediates before oxygen transfer to the aromatic substrate, and (3) are these key intermediates unique to mononuclear nonheme iron dioxygenases?

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Rates of the Phthalate Dioxygenase Reaction with Oxygen Are Dramatically Increased by Interactions with Phthalate and Phthalate Oxygenase Reductase

Cited by 29 publications

References 29 publications

The “Bridging” Aspartate 178 in Phthalate Dioxygenase Facilitates Interactions between the Rieske Center and the Iron(II)−Mononuclear Center

The “Bridging” Aspartate 178 in Phthalate Dioxygenase Facilitates Interactions between the Rieske Center and the Iron(II)−Mononuclear Center

Cytochrome P450 Redox Partner Systems: Biodiversity and Biotechnological Implications

Oxygen activation by mononuclear nonheme iron dioxygenases involved in the degradation of aromatics

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