The Possible Role of Cytochrome P‐450 in the Liver “First Pass Elimination” of a P‐Receptor Blocking Drug

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The use of lidocaine as an oral antiarrhythmic drug is limited by its rapid disposition in the liver. In accordance with this we found that the drug was completely extracted during one passage through the perfused rat liver. The drug binds to rat liver microsomes with a type I spectral change of unusually high affinity. It is rapidly de‐ethylated by the microsomes with an apparent Vmax of about 15 nmol per mg protein × min. The apparent Km for this reaction is about 250 μM. The reaction occurres at about the same rate in isolated rat liver cells. We believe that the high affinity of lidocaine for the cytochrome P‐450 system, as indicated by its type I spectral change, as well as the rapid oxidation of the drug are the two main determinants for the marked liver extraction and first pass effect of the drug.

Section: Discussionsupporting

confidence: 89%

Extraction and Metabolism of Lidocaine in Rat Liver

Nyberg

Karlén

Hedlund

et al. 1977

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“…In the same study the microso-ma1 fraction accounts for most of the rat liver binding capacity. It was suggested that cytochrome-P-450 plays an important role in the presystemic elimination in the rat, which was further supported by studies with cytochrome-P-450 inhibitors in in vitro experimental models (Grundin et al 1974). The presence of several different forms of cytochrome-P-450, rather than a single enzyme with multiple catalytic activities has in recent years been demonstrated by a number of investigators e.g.…”

Section: Discussionmentioning

confidence: 89%

“…Alprenolol is a substrate of the monooxygenase enzyme system in the liver and has a high affinity for cytochrome-P-450 . Based on studies with alprenolol, lidocaine and propranolol, it has been proposed that the presystemic elimination of lipophilic drugs might be due to a cytochrome-P-450-dependent hepatic extraction (Grundin et al 1974). Alprenolol, o-allylphenoxypropanol-isopropylamine is extensively metabo-lized in the rat, dog and man, with aromatic hydroxylation and conjugation with glucuronic acid as the main metabolic pathways (Bodin 1974).…”

mentioning

confidence: 99%

Kinetic Studies of Dose‐Dependent Metabolism of Alprenolol: In Vitro and In Vivo Studies in Different Species

Skånberg

Borg

Fellenius

et al. 1979

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Ahsiract: Kinetic studies of the metabolism of alprenolol were performed with isolated microsomes from the rat, guinea-pig, dog and man at an initial substrate concentration of 0.17-150 pM. In all species the rate of aromatic hydroxylation reached a plateu above 50 pM of alprenolol in contrast to the rate of desisopropylation, where consistent saturation level was not obtained. The Km-values for the aromatic hydroxylation in the guinea-pig and man, 2,7 pM and 1.3 pM respectively, showed no concentration dependency in contrast to the rat (Km, = 0.20 pM, Km, = 26 pM) and the dog (Km, = 0.78 pM, Km, = 66 pM). The apparent Km-value of 0.20 pM for aromatic hydroxylation in the rat seemed to be of the same order of magnitude as reported spectral dissociation constant (Ks = 0.34 pM). In vivo experiments in the rat by oral administration of 7-700 pmol/kg demonstrated a dose-dependent presystemic elimination of alprenolol. The urinary excretion of hydroxy-alprenolol was significantly lower after the highest dose. It is proposed, that the saturation of the aromatic hydroxylation, catalyzed by a high affinity site or subspecies of cytochrome P-450 with a low capacity. contributes to the dose-dependent kinetics in vivo.

“…5 suggest that it is probably also of importance for the low inhibitory effect of alprenolol on oxygen uptake in isolated liver cells. Thus, in the presence of SKF 525-A, which interferes with the binding of alprenolol to cytochrome P-450 (GRUNDIN et al 1974), the inhibitory effect of alprenolol on cellular oxygen uptake is markedly increased. It should be added that SKF 525-A, by itself, in the concentrations used, had no effect on the rate of cellular oxygen uptake.…”

Section: Resultsmentioning

confidence: 99%

The Inhibition of the Mitochondrial NADH Oxidase by Alprenolol and the Protective Effect of Cytochrome P‐450

Grundin

Thor

Orrenius

1975

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The presence of the P-receptor blocking drug alprenolol at a low concentration was found to inhibit markedly the uptake of oxygen catalyzed by liver or heart mitochondria in the presence of P-hydroxybutyrate but not in the presence of succinate. The same was true for the endogenous oxygen uptake by heart slices but not by liver slices or isolated liver cells. In the latter two systems, the rate of oxygen uptake was inhibited only at considerably higher concentrations of the drug. However, in the presence of SKF 525-Awhich prevents the binding of alprenolol to cytochrome P-450liver slices and isolated liver cells were as sensitive as isolated mitochondria to the inhibitory effect on oxygen uptake by alprenolol. Furthermore, liver homogenates or combinations of the liver mitochondria1 and microsomal fractions, in the presence or absence of NADPH, exhibited almost the same sensitivity towards the inhibitory effect of alprenolol on oxygen consumption as the mitochondrial fraction. Thus, the results indicate that alprenolol is a rather potent inhibitor of NADH-linked mitochondria] oxidations, its site of action being localized between NADH and ubiquinone. In the intact liver cell, however, the mitochondria seem to be largely protected from this toxic effect by trapping of the drug by cytochrome P-450. This may in turn be of importance for decreasing the hepatic toxicity of the high concentrations of alprenolol resulting from the efficient liver extraction after oral administration of this drug.