Microsomal prediction of <i>in vivo</i> clearance of CYP2C9 substrates in humans

Carlile, David; Hakooz, Nancy; Bayliss, Martin K.; Houston, J. Brian

doi:10.1046/j.1365-2125.1999.00935.x

Cited by 99 publications

(107 citation statements)

References 42 publications

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“…To minimize nonspecific binding of the substrates to microsomal proteins, lower enzyme concentrations were used in the present study (250 and 125 g/ml for PHT and TLB, respectively), compared with previous reports (Ludden et al, 1997;Carlile et al, 1999). Less than 10% PHT (5 M) and TLB (50 M) was bound to microsomal protein, and the value for TLB was negligible when its concentration reached 1000 M (data not shown).…”

Section: Resultsmentioning

confidence: 78%

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Effect of Albumin on Phenytoin and Tolbutamide Metabolism in Human Liver Microsomes: An Impact More Than Protein Binding

Tang

Lin²,

Rodrigues³

et al. 2002

Drug Metab Dispos

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ABSTRACT:The cytochrome P450 (P450)-dependent conversion of phenytoin (PHT) to p-hydroxy phenytoin (pHPPH), and tolbutamide (TLB) to 4-hydroxy tolbutamide (hydroxy-TLB), in human liver microsomes was studied in the presence of increasing concentrations (0-4%) of bovine serum albumin (BSA). Therefore, the free fraction (f u ) of PHT and TLB varied. Whereas the f u of PHT (5 M) decreased, an increase (3-fold), rather than a decrease in the pHPPH formation rate was observed when BSA (<1%) was present. The stimulation was attributed to a significant decrease in apparent K m . The change, however, was diminished as the BSA concentration reached 4% (PHT f u ‫؍‬ 0.2), in which the reaction velocity remained the same as that measured in the absence of BSA. Therefore, unchanged K m (16.2 ؎ 0.7 M) and V max (9.4 ؎ 0.2 pmol/min/mg of protein) values were determined based on total PHT concentrations, whereas correction for f u led to an unbound K m (K mu ) of ϳ3.2 M. Similarly, the metabolism of TLB (50 M) was enhanced (ϳ2-fold) in the presence of 0.25% BSA but remained only 35% of the control activity (no BSA) at 1% BSA. However, the remaining activity was higher (3-fold) than that determined with an equivalent free concentration of TLB (4 M) calculated according to its f u (0.08). The difference became less significant when BSA concentration was 4% (f u < 0.02). Collectively, the results suggest a 2-fold effect of BSA on PHT and TLB hydroxylation: first, facilitation of the reactions via a decrease in K m ; second, a decrease in f u leading to a drop in reaction rate. For a given P450 reaction, therefore, the effect of BSA may depend upon enzyme affinity, catalytic capacity, and the extent of protein binding.For the longest time, it has been accepted that only unbound drug contributes to pharmacological activities. This free drug hypothesis has also found applications in drug transport, drug metabolism and disposition, receptor binding, enzyme kinetics, and inhibition processes. However, some recent findings appear to contradict this hypothesis. For example, it has been noted that during one passage through the brain, in many cases, more drug than "free drug" can penetrate through the blood-brain barrier (Spector, 2000). Similarly, the hepatic uptake of many lipophilic compounds is not necessarily restricted by protein binding (Kurz and Fichtl, 1983;Pacifici and Viani, 1992), and it has been found that the antifungal activity of itraconazole and ketoconazole is not diminished despite extensive binding albumin (Schäfer-Korting et al., 1995). In agreement, Tran et al. (1997) have reported that the K i value of stiripentol obtained in microsomal studies is more consistent with total plasma concentration than unbound concentration. All these reports suggest that factors, other than protein binding, may be involved in a given biological process.Recently, with the growing demand for quantitative predictions of in vivo pharmacokinetics and drug-drug interactions, this free drug hypothesis has been investigated. For instance, it ...

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Section: Resultsmentioning

confidence: 78%

“…For a better understanding of the effect of protein binding on the estimation of in vitro kinetic parameters, we examined phenytoin (PHT) and tolbutamide (TLB) metabolism in human liver microsomes. These two CYP2C9 substrates are known to differ in terms of protein binding and turnover rates (Bajpai et al, 1996;Carlile et al, 1999). …”

mentioning

confidence: 99%

Effect of Albumin on Phenytoin and Tolbutamide Metabolism in Human Liver Microsomes: An Impact More Than Protein Binding

Tang

Lin²,

Rodrigues³

et al. 2002

Drug Metab Dispos

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“…CL int, in vitro data derived from hepatocyte (Lave et al, 1997a,b;Lau et al, 2002;Shibata et al, 2002;Naritomi et al, 2003) or microsomal incubations (Carlile et al, 1999;Obach, 1999;Naritomi et al, 2001;Andersson et al, 2004) were generated in the authors' laboratory and collated from several published studies (Tables 1-3). Incubation conditions for data generated in the authors' laboratory have been detailed previously (Austin et al, 2002;McGinnity et al, 2004).…”

Section: Methodsmentioning

confidence: 99%

“…Incubation conditions for data generated in the authors' laboratory have been detailed previously (Austin et al, 2002;McGinnity et al, 2004). Data from microsomal studies reflected a variety of methods including formal Michaelis-Menten kinetic analysis [CL int ϭ V max /K m for specific metabolite(s) formation (Carlile et al, 1999;Andersson et al, 2004)] and substrate depletion at low substrate concentrations (Obach, 1999;Naritomi et al, 2001), which was used for all hepatocyte data. Datasets were compiled with several key objectives in mind: to expand existing databases substantially, to provide some assessment of interlaboratory variability, and to complement external datasets in terms of representation from different chemical classes covering a range of physicochemical properties.…”

Section: Methodsmentioning

confidence: 99%

A Unified Model for Predicting Human Hepatic, Metabolic Clearance From in Vitro Intrinsic Clearance Data in Hepatocytes and Microsomes

Riley

McGinnity²,

Austin³

2005

Drug Metab Dispos

328

289

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ABSTRACT:The aim of this study was to evaluate a unified method for predicting human in vivo intrinsic clearance (CL int, in vivo ) and hepatic clearance (CL h ) from in vitro data in hepatocytes and microsomes by applying the unbound fraction in blood (fu b ) and in vitro incubations (fu inc ). Human CL int, in vivo was projected using in vitro data together with biological scaling factors and compared with the unbound intrinsic clearance (CL int, ub, in vivo ) estimated from clinical data using liver models with and without the various fu terms. For incubations conducted with fetal calf serum (n ‫؍‬ 14), the observed CL int, in vivo was modeled well assuming fu inc and fu b were equivalent. CL int, ub, in vivo was predicted best using both fu b Existing methods for the prediction of drug clearance in humans involve the use of in vitro human metabolic stability (intrinsic clearance, CL int ) data (Iwatsubo et al., 1997), consideration of preclinical animal data (Boxenbaum, 1982), or a combination of these approaches (Lave et al., 1997a;Naritomi et al., 2001). In vitro drug metabolism kinetic parameters can provide an estimate of in vivo CL int via "scaling" with established biological scaling factors (SFs) e.g., hepatocellularity for isolated hepatocytes, or a SF for microsomes based on incomplete microsomal recovery from human liver tissue using the cytochrome P450 (P450) content in homogenate and microsomes (Houston, 1984). CL int may subsequently be used to provide an estimate of hepatic clearance (CL h ) using several liver models (Houston, 1984;Ito and Houston, 2004).To date, the more extensive analyses of human clearance predictions have concentrated on P450 substrates, and data have therefore been generated in human liver microsomes (Iwatsubo et al., 1997;Obach, 1999;Naritomi et al., 2001). In general, these studies have been less comprehensive in the range of approaches investigated, with only occasional attention given to chemical class (Obach et al., 1997). Interestingly, these reports have also assessed the ability to predict human CL h rather than the more fundamental parameter, CL int , as advocated initially (Houston, 1984;Ito and Houston, 2004). Some controversy also still exists over use of fu inc , with some laboratories having suggested that fu inc and fu b may cancel, negating their inclusion in liver models (Obach et al., 1997). Recent reports have challenged this assumption (Obach, 1999;Austin et al., 2002) and perhaps suggest that consideration of CL h rather than CL int, in vivo may desensitize such analyses, particularly to errors associated with higher enzyme activities (Ito and Houston, 2004).The aim of this study was to investigate direct in vitro-in vivo scaling of human in vitro data generated in hepatocytes and microsomes for predicting human clearance in vivo by applying recently described models for estimating fu inc (Austin et al., 2002(Austin et al., , 2005. To provide a more mechanistic insight, in vitro human CL int data were compiled from recent in-house and published stud...

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“…This may be partly due to the fact that the contributions of the major metabolic pathways to fibrate clearance have not been systematically investigated. Previous in vitro studies generally focused on a specific pathway by adding either NADPH or UDPGA to initiate oxidative or conjugated reactions [22,29]. Such strategies may hence underestimate the true metabolic rate of fibrates when using in vitro-in vivo extrapolation studies because the contribution of both pathways should not be ignored.…”

Section: Discussionmentioning

confidence: 99%

Metabolism of fibrates by cytochrome P450s and UDP-glycosyltransferases in rat and human liver microsomes

et al. 2012

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Fibrates are widely used for the treatment of dyslipidemia. However, the contributions of the phase I and phase II metabolic pathways to the clearance of fibrates are unclear. In this study, we investigated the metabolism of gemfibrozil (Gem), clofibric acid (CA), fenofibric acid (FA) and bezafibrate (Beza) by cytochrome P450s (P450s) and UDP-glycosyltransferases (UGTs) using a substrate depletion approach. We also compared the metabolic characteristics of rat liver microsomes (RLM) and human liver microsomes (HLM). The intrinsic clearance rates mediated by P450s, UGTs and both were 172 ± 22, 643 ± 26, 798 ± 103 µL min -1 mg -1, respectively, for Gem and 43 ± 11, 88 ± 12, 119 ± 15 µL min -1 mg -1 , respectively, for CA in RLM. The fractions metabolized by P450s and UGTs in RLM were 22% and 81% for Gem, 36% and 74% for CA. The P450-and UGT-mediated depletion rates for Gem were 303 and 1607 nmol min -1 mg -1 in RLM versus 86 and 243 nmol min -1 mg -1 in HLM. The corresponding rates for CA were 1.1 and 1.7 nmol min -1 mg -1 in RLM versus 0.025 and 0.038 nmol min -1 mg -1 in HLM. Accordingly, both P450s and UGTs substantially contribute to the clearance of Gem and CA, with UGTs playing a greater role. To avoid under-estimating the impact of these pathways, it is necessary to measure NADPH-and UDPGA-dependent metabolism. Although the fractions of these two pathways in RLM and HLM were similar, the depletion rate of Gem and CA in RLM was higher than that in HLM. The metabolism of FA and Beza by P450s and UGTs was too low to calculate intrinsic clearance in both RLM and HLM. These results indicate that fibrates are metabolized via similar pathways in rats and humans, and it is applicable to use RLM to predict the clearance of fibrates in human.

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Microsomal prediction of in vivo clearance of CYP2C9 substrates in humans

Cited by 99 publications

References 42 publications

Effect of Albumin on Phenytoin and Tolbutamide Metabolism in Human Liver Microsomes: An Impact More Than Protein Binding

Effect of Albumin on Phenytoin and Tolbutamide Metabolism in Human Liver Microsomes: An Impact More Than Protein Binding

A Unified Model for Predicting Human Hepatic, Metabolic Clearance From in Vitro Intrinsic Clearance Data in Hepatocytes and Microsomes

Metabolism of fibrates by cytochrome P450s and UDP-glycosyltransferases in rat and human liver microsomes

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