The Stoichiometry of the Cytochrome P-450-catalyzed Metabolism of Methoxyflurane and Benzphetamine in the Presence and Absence of Cytochrome b5

Gruenke, Larry D.; Konopka, Krystyna; Cadieu, Marie; Waskell, Lucy

doi:10.1074/jbc.270.42.24707

Cited by 86 publications

(92 citation statements)

References 67 publications

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“…Wild type cyt b 5 caused a 6-fold stimulation of the rate of fluoride formation from 0.21 Ϯ 0.03 nmol of F Ϫ min Ϫ1 nmol of cyt P450 Ϫ1 in the absence of cyt b 5 to 1.23 Ϯ 0.2 nmol min Ϫ1 nmol of cyt P450 Ϫ1 with cyt b 5 . These results are similar to the rate of methoxyflurane metabolism observed in previous studies (7,9). Replacing the conserved residues Pro 95 and Lys 94 with alanines and reversing the amino acid sequence of the linker region did not significantly alter the rate of F Ϫ formation.…”

Section: Construction and Expression Of Mutant Cyts B 5 With Linker Rsupporting

confidence: 79%

“…It is unlikely that mutation of the cyt b 5 linker region alters the relative formation of the two products, as recent modeling studies have shown that, in cyt P450 2E1, the preferential metabolism of methoxyflurane to methoxydifluroacetic acid is the result of differences in the relative activation energy required for H atom extraction rather than favorable substrate binding conformations (31). In addition, the relative amounts of methoxyflurane products formed by cyt P450 2B4 are the same in the presence and absence of cyt b 5 (7). These studies indicate that the observed reduction in F Ϫ formation caused by mutation of the cyt b 5 linker region is the result of an attenuation in the overall metabolism of methoxyflurane rather than a selective decrease in O-demethylation relative to dechlorination.…”

Section: Construction and Expression Of Mutant Cyts B 5 With Linker Rmentioning

confidence: 61%

“…5 -The method used to measure the rate of methoxyflurane metabolism by cyt P450 2B4 in the presence and absence of cyt b 5 is a modification of a previously described procedure (7). The reaction components were added to a reaction mixture in a specific sequence: 50 mM KPO 4 , pH 7.4, 10 M cyt P450 2B4, 10 M cyt P450 reductase, 0 -90 M cyt b 5 , and 1.9 mM DLPC.…”

Section: Methodsmentioning

confidence: 99%

“…However, cyt b 5 can also inhibit the rate of oxidation catalyzed by cyt P450, by competing with cyt P450 reductase. This effect of cyt b 5 is observed as a decrease in the overall rate of NADPH consumption (7).…”

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confidence: 99%

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The role of the length and sequence of the linker domain of cytochrome b5 in stimulating cytochrome P450 2B4 catalysis.

Clarke

Bidwai

et al. 2004

Journal of Biological Chemistry

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Cytochrome b 5 (cyt b 5 ) is a 15-kDa amphipathic protein with a cytosolic amino-terminal catalytic heme domain, which is anchored to the microsomal membrane by a hydrophobic transmembrane ␣-helix at its carboxyl terminus. These two domains are connected by an ϳ15-amino acid linker domain, Ser 90 -Asp 104 , which has been modified by site-directed mutagenesis to investigate whether the length or sequence of the linker influences the ability of cyt b 5 to bind ferric cytochrome P450 2B4 and donate an electron to oxyferrous (cyt P450 2B4), thereby stimulating catalysis. Because shortening the linker by 8 or more amino acids markedly inhibited the ability of cyt b 5 to bind cyt P450 2B4 and stimulate catalysis by this isozyme, it is postulated 7 amino acids are sufficient to allow a productive interaction. All mutant cyts b 5 except the protein lacking the entire 15-amino acid linker inserted normally into the microsomal membrane. Alternatively, lengthening the linker by 16 amino acids, reversing the sequence of the amino acids in the linker, and mutating conserved linker residues did not significantly alter the ability of cyt b 5 to interact with cyt P450 2B4. A model for the membranebound cyt b 5 -cyt P450 complex is presented.Microsomal cytochrome b 5 (cyt b 5 ) 1 is an amphipathic electron transfer hemoprotein located in the membrane of the endoplasmic reticulum. It provides electrons for a broad range of reactions, including fatty acid desaturation, cholesterol biosynthesis, and a variety of cytochrome P450-dependent oxidation and hydroxylation reactions (1, 2).Cytochrome P450 (cyt P450) is responsible for the oxidation of a large number of substrates. The overall stoichiometry of the reaction catalyzed by cyt P450 is shown in Reaction 1, where RH is the substrate (3).The cyt P450 catalytic reaction occurs via a reaction cycle that involves substrate binding, reduction of the ferric heme, O 2 binding, reduction of the oxyferrous heme (second electron transfer), substrate oxidation, and finally product dissociation (4). Both ferric and oxyferrous cyt P450 receive electrons from NADPH via its redox partner, NADPH-cytochrome P450 reductase (cyt P450 reductase), whereas cyt b 5 can donate the second electron. Because of the high redox potential of Х20 mV for cyt b 5 , the first electron required to reduce cyt P450 from the ferric to the ferrous state is always transferred from NADPH via cyt P450 reductase. However, as the redox potential of cyt P450 increases from ХϪ230 mV to ϩ50 mV on transition to the oxyferrous state, the second electron can be obtained from either cyt P450 reductase or cyt b 5 (5, 6).Depending on the substrate, isozyme of cyt P450 and the experimental conditions cyt b 5 can stimulate, inhibit, or have no effect on cyt P450 activity (2). Studies of the stoichiometry of the metabolism of benzphetamine and methoxyflurane by cyt P450 2B4 have shown that cyt b 5 increases the efficiency of catalysis by cyt P450 2B4 primarily by decreasing the formation of the side-product superoxide. However, cyt b...

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Section: Construction and Expression Of Mutant Cyts B 5 With Linker Rsupporting

confidence: 79%

Section: Construction and Expression Of Mutant Cyts B 5 With Linker Rmentioning

confidence: 61%

Section: Methodsmentioning

confidence: 99%

mentioning

confidence: 99%

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The role of the length and sequence of the linker domain of cytochrome b5 in stimulating cytochrome P450 2B4 catalysis.

Clarke

Bidwai

et al. 2004

Journal of Biological Chemistry

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“…Some of the products formed by these enzymes have also been implicated as causative agents in a number of cancers (Gonzales & Gelboin, 1994;Shimada et al, 1996). Intermediates involved in dioxygen activation have been proposed (Fruetel et al, 1992, Gruenke et al, 1995, Loida & Sligar, 1993 from the production of superoxide or peroxide upon loss of catalytic efficiency. The mechanism of dioxygen activation is the least understood step in P450 catalysis (Figure 1), which begins with the reduction of the dioxygen complex (oxy-P450, 4 in Figure 1).…”

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confidence: 99%

Reduced Oxy Intermediate Observed in D251N Cytochrome P450_cam

1997

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Cytochrome P450s are ubiquitous heme proteins responsible for various oxidative metabolic processes. The overall rate-determining step in the catalytic cycle of native cytochrome P450 cam is the reduction of the dioxygen complex, which has made detection of catalytic intermediates after this reduction impossible. However, for the site-specific mutant D251N cytochrome P450 cam (which affects proton transfer near the catalytic center), the overall rate-determining step occurs after the reduction of oxy-P450. As a consequence, we have observed in the UV-visible spectrum during catalytic turnover a new intermediate that is one electron reduced from oxy-P450 with an intact dioxygen bond.

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Identification and circumvention of bottlenecks in CYP21A2‐mediated premedrol production using recombinant Escherichia coli

König

Brixius‐Anderko

Milhim

et al. 2019

Biotech & Bioengineering

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Synthetic glucocorticoids such as methylprednisolone are compounds of fundamental interest to the pharmaceutical industry as their modifications within the sterane scaffold lead to higher inflammatory potency and reduced side effects compared with their parent compound cortisol. In methylprednisolone production, the complex chemical hydroxylation of its precursor medrane in position C21 exhibits poor stereo‐ and regioselectivity making the process unprofitable and unsustainable. By contrast, the use of a recombinant E. coli system has recently shown high suitability and efficiency. In this study, we aim to overcome limitations in this biotechnological medrane conversion yielding the essential methylprednisolone‐precursor premedrol by optimizing the CYP21A2‐based whole‐cell system on a laboratory scale. We successfully improved the whole‐cell process in terms of premedrol production by (a) improving the electron supply to CYP21A2; here we use the N‐terminally truncated version of the bovine NADPH‐dependent cytochrome P450 reductase (bCPR−27) and coexpression of microsomal cytochrome b5; (b) enhancing substrate access to the heme by modification of the CYP21A2 substrate access channel; and (c) circumventing substrate inhibition which is presumed to be the main limiting factor of the presented system by developing an improved fed‐batch protocol. By overcoming the presented limitations in whole‐cell biotransformation, we were able to achieve a more than 100% improvement over the next best system under equal conditions resulting in 691 mg·L−1·d−1 premedrol.

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The Stoichiometry of the Cytochrome P-450-catalyzed Metabolism of Methoxyflurane and Benzphetamine in the Presence and Absence of Cytochrome b5

Cited by 86 publications

References 67 publications

The role of the length and sequence of the linker domain of cytochrome b5 in stimulating cytochrome P450 2B4 catalysis.

The role of the length and sequence of the linker domain of cytochrome b5 in stimulating cytochrome P450 2B4 catalysis.

Reduced Oxy Intermediate Observed in D251N Cytochrome P450_cam

Identification and circumvention of bottlenecks in CYP21A2‐mediated premedrol production using recombinant Escherichia coli

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The Stoichiometry of the Cytochrome P-450-catalyzed Metabolism of Methoxyflurane and Benzphetamine in the Presence and Absence of Cytochrome b5

Cited by 86 publications

References 67 publications

The role of the length and sequence of the linker domain of cytochrome b5 in stimulating cytochrome P450 2B4 catalysis.

The role of the length and sequence of the linker domain of cytochrome b5 in stimulating cytochrome P450 2B4 catalysis.

Reduced Oxy Intermediate Observed in D251N Cytochrome P450cam

Identification and circumvention of bottlenecks in CYP21A2‐mediated premedrol production using recombinant Escherichia coli

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Product

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Reduced Oxy Intermediate Observed in D251N Cytochrome P450_cam