Saturable Uptake of Lipophilic Amine Drugs into Isolated Hepatocytes: Mechanisms and Consequences for Quantitative Clearance Prediction

Hallifax, David; Houston, J. Brian

doi:10.1124/dmd.107.015131

Cited by 66 publications

(70 citation statements)

References 46 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…After appropriate binding corrections, more potent hepatocyte inhibition (as evident by lower K i values) would suggest the involvement of hepatic transporters because a higher concentration of unbound drug available for enzyme inhibition can be achieved compared with a similar incubation concentration in microsomes (Ito et al, 1998). Alternatively, similar values would indicate that any hepatic accumulation results from intracellular binding or lysosomal trapping (Grime and Riley, 2006;Hallifax and Houston, 2007). We recently demonstrated good concordance between K i values (range 0.05-30 M) determined in rat hepatic microsomes and freshly isolated hepatocytes using seven P450 inhibitors (fluconazole, fluoxetine, fluvoxamine, ketoconazole, miconazole, omeprazole, and quinine) with a range of uptake properties (cell/medium concentration ratios 4 -6000).…”

Section: Introductionmentioning

confidence: 98%

Comparative Use of Isolated Hepatocytes and Hepatic Microsomes for Cytochrome P450 Inhibition Studies: Transporter-Enzyme Interplay

Brown¹,

Wilby²,

Alder³

et al. 2010

Drug Metab Dispos

Self Cite

View full text Add to dashboard Cite

ABSTRACT:Accurate assignment of the concentration of victim drug/inhibitor available at the enzyme active site, both in vivo and within an in vitro incubation, is an essential requirement in rationalizing and predicting drug-drug interactions. Inhibitor accumulation within the liver, whether as a result of active transport processes or intracellular binding, may best be accounted for using hepatocytes rather than hepatic microsomes to estimate in vitro inhibitory potency. The aims of this study were to compare K i values determined in rat liver microsomes and freshly isolated rat hepatocytes of four cytochrome P450 (P450) inhibitors (clarithromycin, enoxacin, nelfinavir, and saquinavir) with known hepatic transporter involvement and a range of uptake (cell/medium concentration ratios 20-3000) and clearance (10-1200 l/min/10 6 cells) properties.Inhibition studies were performed using two well established P450 probe substrates (theophylline and midazolam). Comparison of unbound K i values showed marked differences between the two in vitro systems for inhibition of metabolism. In two cases (clarithromycin and enoxacin, both low-clearance drugs), inhibitory potency in hepatocytes markedly exceeded that in microsomes (10-to 20-fold), and this result was consistent with their high cell/medium concentration ratios. For nelfinavir and saquinavir (high-clearance, extensively metabolized drugs), the opposite trend was seen in the K i values: despite very high cell/medium concentration ratios, stronger inhibition was evident within microsomal preparations. Hence, the consequences of hepatic accumulation resulting from uptake transporters vary according to the clearance of the inhibitor. This study demonstrates that transporter-enzyme interplay can result in differences in inhibitory potency between microsomes and hepatocytes and hence drug-drug interaction predictions that are not always intuitive.

show abstract

Section: Introductionmentioning

confidence: 98%

Comparative Use of Isolated Hepatocytes and Hepatic Microsomes for Cytochrome P450 Inhibition Studies: Transporter-Enzyme Interplay

Brown¹,

Wilby²,

Alder³

et al. 2010

Drug Metab Dispos

Self Cite

View full text Add to dashboard Cite

show abstract

“…where K a represents microsomal protein binding affinity, P the microsomal protein concentration (mg/ml), K p the hepatocyte/medium concentration ratio, and V R a V cell /V inc ratio, where V cell is the cell volume and V inc the incubation volume (Brown et al, 2007b;Hallifax and Houston, 2007). V R is 0.005 at the cell concentration of 10 6 cells/ml (Brown et al, 2007b).…”

Section: Methodsmentioning

confidence: 99%

“…A database of 39 drugs and their corresponding fu mic and fu hep values was collated either from in house data or from the literature (Austin et al, 2002(Austin et al, , 2005Brown et al, 2007a;Hallifax and Houston, 2007). In the aforementioned studies, different methods were used to determine the drug binding in hepatocyte incubations, namely oil centrifugation (using live cells), dialysis (using dead cells), and ultrafiltration (using dead cells).…”

Section: Methodsmentioning

confidence: 99%

mentioning

confidence: 99%

“…The authors proposed a linear 1:1 relationship between microsomal and hepatocyte binding for incubations of 1 mg/ml and 10 6 cells/ml, respectively, indicating that the fu hep can be extrapolated from microsomal studies. However, the applicability of this correlation has been questioned because of the small number of compounds investigated (Hallifax and Houston, 2007).To further explore the relationship between binding in microsomal and hepatocyte systems, a detailed analysis was carried out involving 39 drugs. A nonlinear empirical equation is proposed as an alternative to the linear relationship to relate binding between the two systems.…”

mentioning

confidence: 99%

See 2 more Smart Citations

Hepatocellular Binding of Drugs: Correction for Unbound Fraction in Hepatocyte Incubations Using Microsomal Binding or Drug Lipophilicity Data

Kilford

Gertz²,

Houston³

et al. 2008

Drug Metab Dispos

Self Cite

138

View full text Add to dashboard Cite

The need to incorporate the fraction unbound in microsomes (fu mic ) to obtain meaningful drug concentrations for the prediction of intrinsic clearance and cytochrome P450 inhibition potential is widely accepted (Obach, 1996;Ito and Houston, 2005;Rostami-Hodjegan and Tucker, 2007). Recently, two equations based on drug lipophilicity have been developed for prediction of fu mic (Austin et al., 2002;Hallifax and Houston, 2006) that avoid experimental determinations. The limitations of these empirical predictive tools and their applicability for fu mic predictions over a range of lipophilicity and microsomal protein concentrations have been addressed (Gertz et al., 2008).Analogous to applying a correction for microsomal drug binding to in vitro clearance and inhibition parameters, it is important that the fraction unbound in hepatocyte incubations (fu hep ) is also considered for in vitro-in vivo extrapolation (McGinnity et al., 2006;Brown et al., 2007b). However, this need has yet to be broadly applied, perhaps due to the lack of comprehensive demonstration of its value. In a recent study by Austin et al. (2005), the extent of binding between the microsomal and hepatocyte incubations was compared using hepatocyte data (n ϭ 14) and the corresponding fu mic from a previous study (Austin et al., 2002). The authors proposed a linear 1:1 relationship between microsomal and hepatocyte binding for incubations of 1 mg/ml and 10 6 cells/ml, respectively, indicating that the fu hep can be extrapolated from microsomal studies. However, the applicability of this correlation has been questioned because of the small number of compounds investigated (Hallifax and Houston, 2007).To further explore the relationship between binding in microsomal and hepatocyte systems, a detailed analysis was carried out involving 39 drugs. A nonlinear empirical equation is proposed as an alternative to the linear relationship to relate binding between the two systems. In addition, prediction of fu hep directly from the logP/D metric is assessed over a wide range of lipophilicity (Ϫ0.13 to 5.93). The implications of these findings on the estimation of hepatocellular drug concentration for intrinsic clearance and inhibition parameter predictions are discussed. Materials and MethodsA database of 39 drugs and their corresponding fu mic and fu hep values was collated either from in house data or from the literature (Austin et al., 2002(Austin et al., , 2005Brown et al., 2007a;Hallifax and Houston, 2007). In the aforementioned studies, different methods were used to determine the drug binding in hepatocyte incubations, namely oil centrifugation (using live cells), dialysis (using dead cells), and ultrafiltration (using dead cells). Microsomal and hepatocyte binding are defined by eqs. 1 and 2, respectively: ABBREVIATIONS: fu mic , fraction unbound in microsomes; fu hep , fraction unbound in hepatocyte incubations; K a , microsomal protein binding affinity; K p , hepatocyte/medium concentration ratio; V R , ratio of the cell and incubation volume; logP/D...

show abstract

Fluvoxamine vs Placebo and Clinical Deterioration in Outpatients With Symptomatic COVID-19

Lenze

Mattar

Zorumski

et al. 2020

JAMA

464

562

View full text Add to dashboard Cite

Key PointsQuestionDoes fluvoxamine, a selective serotonin reuptake inhibitor and σ-1 receptor agonist, prevent clinical deterioration in outpatients with acute coronavirus disease 2019 (COVID-19)?FindingsIn this randomized trial that included 152 adult outpatients with confirmed COVID-19 and symptom onset within 7 days, clinical deterioration occurred in 0 patients treated with fluvoxamine vs 6 (8.3%) patients treated with placebo over 15 days, a difference that was statistically significant.MeaningIn this preliminary study, adult outpatients with symptomatic COVID-19 treated with fluvoxamine, compared with placebo, had a lower likelihood of clinical deterioration over 15 days; however, determination of clinical efficacy would require larger randomized trials with more definitive outcome measures.

show abstract

Saturable Uptake of Lipophilic Amine Drugs into Isolated Hepatocytes: Mechanisms and Consequences for Quantitative Clearance Prediction

Cited by 66 publications

References 46 publications

Comparative Use of Isolated Hepatocytes and Hepatic Microsomes for Cytochrome P450 Inhibition Studies: Transporter-Enzyme Interplay

Comparative Use of Isolated Hepatocytes and Hepatic Microsomes for Cytochrome P450 Inhibition Studies: Transporter-Enzyme Interplay

Hepatocellular Binding of Drugs: Correction for Unbound Fraction in Hepatocyte Incubations Using Microsomal Binding or Drug Lipophilicity Data

Fluvoxamine vs Placebo and Clinical Deterioration in Outpatients With Symptomatic COVID-19

Contact Info

Product

Resources

About