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ABSORPTION, DISTRIBUTION, METABOLISM, AND EXCRETION
Division of Drug Delivery and Disposition, School of Pharmacy, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina
Received January 22, 2003; accepted April 3, 2003.
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Abstract |
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 Top Abstract Materials and MethodsResultsDiscussionReferences |
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55%,
whereas there was only 12% inhibition of P-gp-mediated efflux of
quinidine at that rifampin dose. Coperfusion of rifampin at a concentration of
500 µM abolished P-gp-mediated efflux of verapamil at the BBB. However,
only 40% inhibition of P-gp-mediated efflux of quinidine was observed
with coperfusion of rifampin, even at a 2-fold higher rifampin concentration
(1000 µM). The present studies demonstrate that P-gp function at the BBB
can be modulated by rifampin in a dose- and concentration-dependent manner.
The degree to which rifampin inhibits P-gp-mediated transport is dependent on
the substrate molecule.
).
In humans, only the MDR1 gene-encoded P-gp is capable of conveying
resistance to a large number of compounds, whereas in rodents the drug
transport function is shared between mdr1a and mdr1b
(Thiebaut et al., 1987;
Hsu et al., 1989). In
contrast, the MDR2 gene encodes a phospholipid transporter, the
involvement of which in drug absorption or disposition is unclear
(Smit et al., 1993;
Ruetz and Gros, 1994).
The importance of P-gp was first recognized with the occurrence of
multidrug resistance during chemotherapy
(Juliano and Ling, 1976).
Tumor cells are protected against various cytotoxic agents due to
overexpression of P-gp; the transporter reduces intracellular concentrations
of P-gp substrates such as vinca alkaloids, anthracyclines, and taxol
(Leveille-Webster and Arias,
1995). It is becoming increasingly clear that expression of P-gp
in normal tissues plays an important role in the disposition and
pharmacological activity of a broad range of compounds. P-gp is expressed
constitutively in the epithelial cells lining the luminal surface of many
organs associated with excretory or barrier functions, i.e., the hepatic bile
canalicular membrane, the renal proximal tubule, and the villus-tip enterocyte
in the small intestine. In addition, P-gp is expressed in the endothelial
cells that comprise the blood-brain barrier (BBB) and blood-testes barrier
(Cordon-Cardo et al., 1989).
The expression of P-gp in these tissues associated with drug absorption,
distribution to sites of biological activity, and elimination from the body
has led to the hypothesis that P-gp evolved as a protective mechanism against
a wide range of potentially toxic substances, serving to limit distribution
and facilitate elimination of substrates
(Schinkel, 1997;
Ambudkar et al., 1999).
Since the discovery of the drug efflux activity of P-gp, numerous attempts
have been made to inhibit P-gp-mediated drug efflux. Initial investigations
used existing compounds, such as calcium channel blockers (e.g., verapamil),
immunosuppressive agents (e.g., cyclosporine A), and antiarrhythmic drugs
(e.g., quinidine). However, because of undesirable pharmacological effects or
limited in vivo inhibition of transport, more specific and potent
"second-generation" P-gp modulators have been developed, such as
the acridone carboxamide GF120918 (Hyafil
et al., 1993) and a nonimmunosuppressive analog of cyclosporin A,
PSC833 (Lemaire et al.,
1996).
Several recent studies have shown that P-gp expression can be up-regulated
in normal tissues as well as in tumor cells. Morphine increased P-gp content
approximately 2-fold in rat brain after a 5-day treatment
(Aquilante et al., 2000). The
immunosupressant cyclosporine A has been shown to increase P-gp in both liver
and intestine (Prince et al.,
1996). Rifampin was able to induce P-gp in both in vivo studies in
humans (Greiner et al., 1999)
and in vitro in human colon carcinoma cells
(Schuetz et al., 1996).
Dexamethasone rapidly increased P-gp expression more than 4.5- and 2-fold in
rat liver and lung, respectively, whereas P-gp expression was decreased 40% in
kidney (Demeule et al.,
1999).
Based on the broad substrate specificity and tissue distribution of P-gp,
modulation of P-gp activity may result in significant alterations in the
pharmacokinetics and, potentially, the pharmacodynamics of P-gp substrates.
For example, the brain/blood distribution ratio of the opioid peptide
[D-Pen2,5]-enkephalin was increased 4-fold, and the
EC50 was decreased 10-fold, in mdr1a(–/–)
mice compared with FVB controls (Chen and
Pollack, 1998). Similarly, mdr1a(–/–) mice
evidenced enhanced brain accumulation and antinociceptive effect of morphine
compared with their gene-competent counterparts
(Zong and Pollack, 2000).
Although not as well studied, induction of P-gp in normal tissue also is
likely to be of clinical importance. For example, P-gp induction in response
to rifampin administration was implicated in the reduced pharmacodynamic
response to morphine in a study of 10 healthy human volunteers
(Fromm et al., 1997).
Similarly, induction of P-gp has been proposed as a possible mechanism of
resistance to antiretroviral agents (Lee
et al., 1998).
Although several experiments have shown that modulation of P-gp activity can influence drug disposition and action, the dynamics of P-gp modulation have yet to be addressed, especially with respect to the impact on BBB transport per se. The present studies were designed to evaluate modulation of P-gp transport activity in the murine BBB using an in situ brain perfusion model.
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Materials and Methods |
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TopAbstractMaterials and MethodsResultsDiscussionReferences |
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Animals. Adult CF-1 mice [mdr1a(–/–) and mdr1a(+/+), 30–45 g] were purchased from Charles River Laboratories, Inc. (Wilmington, MA) and maintained in a breeding colony in the School of Pharmacy (The University of North Carolina, Chapel Hill, Chapel Hill, NC). Animals were housed in a temperature- and humidity-controlled room with a 12-h light/dark cycle and had free access to food and water. The experimental protocol was approved by the Institutional Animal Care and Use Committee of the University of North Carolina at Chapel Hill. All experimental procedures were conducted according to the Guide for the Care and Use of Laboratory Animals (Institute of Laboratory Animal Resources, Commission on Life Sciences, National Research Council, Washington, DC, 1996).
Induction of P-gp Expression by Morphine and Rifampin in Mice. Morphine [10, 20, and 30 mg/kg s.c. three times/day on days 1, 2, and 3, respectively; saline (10 µl/g) as a control] or rifampin [200 mg/kg i.p. once daily for 4 days; DMSO (4 µl/g) as a control] was administered to CF-1 mice [mdr1a(–/–) and mdr1a(+/+), n = 3/group, 35–45 g]. After a 24-h washout, animals were decapitated and brain samples were harvested. Western blot analysis was performed to assess P-gp expression in the brain.
In a separate experiment, CF-1 mice [mdr1a(+/+), n = 4/group, 35–45 g] were pretreated with rifampin (200 mg/kg/day i.p.) or DMSO (4 µl/g) for 4 days. After a 24-, 48-, or 72-h washout, mice were anesthetized and prepared for brain perfusion as described below to assess P-gp function in the BBB using brain uptake of verapamil as an index of P-gp function. Mice receiving an acute dose of rifampin (200 mg/kg i.p.) 2 h before perfusion also were included in the P-gp functional test.
Inhibition of P-gp in the BBB by Pretreating Mice with a Single Dose of Rifampin. The results of the preceding experiment indicated that any induction of BBB P-gp that might have occurred in response to rifampin pretreatment was masked by concomitant P-gp inhibition. To further evaluate the dynamics of the inhibitory process, mdr1a(+/+) CF-1 mice (30–45 g, n = 4/group) were pretreated with rifampin (50, 75, 100, and 150 mg/kg i.p.). P-gp-deficient animals received a 100 mg/kg i.p. dose of rifampin to control for any nonspecific effects of rifampin on processes other than P-gp-mediated efflux, and DMSO (4 µl/g) was administered as a vehicle control. At 1 h postdose, mice were anesthetized and prepared for brain perfusion to assess P-gp function. In this experiment, the brain uptake of both verapamil and quinidine was used as independent indices of P-gp activity. A blood sample was obtained at the time of perfusion to determine the circulating concentration of rifampin to develop relationships between transport inhibition and rifampin concentration.
Inhibition of P-gp-Mediated Efflux of Verapamil and Quinidine by Coperfusion with Rifampin. CF-1 mice (30–45 g, n = 4/group) were anesthetized and prepared for brain perfusion. Verapamil and quinidine brain uptake was measured to assess P-gp function during coperfusion with differing concentrations of rifampin (50, 200, and 500 µM for verapamil; 500 and 1000 µM for quinidine).
Inhibition of P-gp-Mediated Efflux of Quinidine by Coperfusion with Verapamil. CF-1 mice (30–45 g, n = 4/group) were anesthetized and prepared for brain perfusion. Quinidine brain uptake was measured to examine P-gp function during coperfusion with various concentrations of verapamil (50, 200, and 1000 µM).
Western Blot Analysis. Freshly isolated brain tissue was processed
to obtain membrane homogenate using a procedure modified from the method of
Bergwerk et al. (1996).
Briefly, brain tissue was rinsed and homogenized with a glass dounce in 4
volumes (w/v) of buffer A (1 mM NaHCO3 and 50 µM
phenylmethylsulfonyl fluoride) at 4°C. The homogenate was diluted to a
final volume of 10.6 ml/g brain with addition of buffer B (buffer A with 1 mM
EDTA). Aliquots (1.5 ml) of the homogenate then were extracted with 30 ml of
buffer C (0.1 M Na2CO3, 50 µM phenylmethylsulfonyl
fluoride, 1 µg/ml aprotinin, and 1 µg/ml leupeptin) at 4°C for 15
min, followed by centrifugation at 100,000g for 1 h. The resulting
pellet was reconstituted in buffer C. Protein content of the membrane
preparations was determined by the method of Lowry et al.
(1951). Plasma membrane
preparations were resuspended in NuPAGE sample buffer and aliquots (20 µl)
of sample (30 µg of protein) were loaded in triplicate onto a 4 to 12%
NuPAGE Bis-Tris gel. Plasma membrane preparations from P-gp-overexpressing
intestinal cells were used as a positive control. SDS-PAGE electrophoresis was
conducted on ice for 2 h at 160 V (constant) under reducing conditions. After
electrophoresis, the samples were transferred onto polyvinylidene difluoride
membranes for 1 h at 25 V (constant). Nonspecific binding sites were blocked
with 5% nonfat dry milk in TBS-Tween 0.05% after an overnight transfer. The
membranes were incubated with P-gp antibody mdr(Ab-1) (rabbit IgG, 1:1500
dilution) (Oncogene Science, Cambridge, MA) in TBS-Tween for 1 h. The
membranes then were washed with TBS-Tween (3 x 10 min) and incubated
with a horse-radish peroxidase-linked goat anti-rabbit antibody (1:3000
dilution) in TBS-Tween for 1 h, followed by rinsing with TBS-Tween (3 x
10 min). The membrane was exposed to Amersham ECL detection agent, and band
intensity was determined by densitometric analysis.
In Situ Mouse Brain Perfusion. CF-1 mice [mdr1a(+/+) and
mdr1a(–/–), 30–45 g, n = 4/group] were
prepared for in situ brain perfusion according to the method of Dagenais et
al. (2000). Briefly, mice were
anesthetized with ketamine/xylazine (140/8 mg/kg i.p.) and the right common
carotid artery was catheterized (polyethylene tubing, 0.30 mm i.d. x
0.70 mm o.d.) after ligation of the external branch. The cardiac ventricles
were severed immediately before brain perfusion with Krebs-bicarbonate buffer
via a syringe pump (60 s, 2.5 ml/min, pH 7.4 with 95% O2 and 5%
CO2, 37°C) containing 1 µM [ldqb]3H]verapamil
(0.1 µCi/ml) or 1 µM [3H]quinidine (0.15 µCi/ml).
[14C]inulin (0.3 µCi/ml) was added as a vascular space marker.
The perfusion was terminated by decapitation and the brain was dissected on
ice. The right hemisphere (140 mg) and perfusate (150 mg) were
collected and weighed in tared 8-ml glass scintillation vials. Brain tissue
was digested with 0.7 ml of Solvable (PerkinElmer Life Sciences) at 50°C
overnight. Samples were mixed with 5 ml of scintillation cocktail (Ultimate
Gold; PerkinElmer Life Sciences). Total radioactivity (3H and
14C) was determined simultaneously in a PerkinElmer 1600TR liquid
scintillation analyzer.
Quantitation of Rifampin by HPLC. All samples were stored at –20°C before analysis. Rifampin concentrations in serum were determined by reversed-phase capillary HPLC with UV detection (Agilent 1100 series). After addition of internal standard (sulindac, 10 µl of a 1 mg/ml solution) to the serum sample (50 µl), acetonitrile (100 µl) was added to precipitate proteins (centrifugation at 14,000 rpm for 3 min). The supernatant then was evaporated to dryness under nitrogen and reconstituted in 100 µl of mobile phase [acetonitrile/5 mM ammonium acetate, pH 4.0, 38:62 (v/v)], of which 10 µl was injected onto the HPLC. Chromatographic separation was achieved on a Zorbax C8 column (1 x 150 mm, particle size 5 µm) under isocratic conditions (50 µl/min). The absorbance of column eluent was monitored at 254 nm. Standard curve was linear between 1.6 and 200 µg/ml when 50 µl of serum was extracted.
Calculation of BBB Transport Parameters. Parameters related to the
in situ brain perfusion were calculated based on the method described by Smith
(1996). Brain vascular volume
(Vvasc, ml/100 g) was estimated from tissue distribution
of lsqb]14C]inulin, which is known to diffuse very slowly across
the BBB, according to the following equation:
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):
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Data Analysis. Data are presented as mean ± S.D. Student's t test or analysis of variance, where appropriate, were used to determine the statistical significance of difference between experimental groups. Statistical significance was defined as p < 0.05.
The degree of inhibition of P-gp-mediated efflux of verapamil or quinidine
was defined as follows:
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The concentration-dependent inhibition of P-gp-mediated verapamil or
quinidine efflux data were analyzed by nonlinear least regression (WinNonlin
3.2; Pharsight, Mountain View, CA):
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is the sigmoidicity factor. |
Results |
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TopAbstractMaterials and MethodsResultsDiscussionReferences |
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Functional Evaluation of P-gp after Multiple-Dose Rifampin Pretreatment. The initial brain uptake clearance (CLup) of verapamil in mice after pretreatment with rifampin is shown in Fig. 2. Unexpectedly, verapamil CLup was significantly higher (consistent with inhibition, rather than induction, of P-gp-mediated transport) 24 h after treatment in rifampin-treated mice compared with controls. The effect of rifampin was not entirely diminished until 72 h after the last rifampin dose. Further study with an acute rifampin dose (200 mg/kg i.p.) indicated a significant inhibitory effect of rifampin on P-gp function in the BBB.
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Dose-Dependent Inhibition of P-gp by Rifampin. Single-dose rifampin treatment increased both verapamil and quinidine initial brain uptake in mdr1a(+/+) mice in a dose-dependent manner (Fig. 3). Rifampin was much less potent in inhibiting of P-gp-mediated quinidine efflux compared with verapamil efflux. Maximum inhibition of P-gp-mediated efflux of verapamil by rifampin was approximately 55% [with 100% inhibition defined as uptake in mdr1a(–/–) mice], whereas there was only about 12% inhibition of P-gp-mediated efflux of quinidine at the highest rifampin dose tested. A 100-mg/kg dose of rifampin produced no effect on brain uptake of verapamil or quinidine in mdr1a(–/–) mice compared with the DMSO-treated controls (p > 0.05). As was the case for the dose-response profile, the relationship between percentage of inhibition of quinidine efflux and rifampin blood concentration also was shifted rightward compared with that of verapamil efflux (Fig. 4).
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Influence of Rifampin Coperfusion on Brain Uptake of Verapamil and Quinidine. Coperfusion of rifampin resulted in a concentration-dependent increase in verapamil uptake clearance in mdr1a(+/+) mice (Fig. 5). The apparent IC50 value for inhibition by rifampin was about 220 µM. Rifampin at a concentration of 500 µM was able to inhibit almost completely P-gp-mediated efflux of verapamil in the BBB [verapamil CLup of 120 ± 41 ml/100 g/min in rifampin-treated mdr1a(+/+) mice versus 136 ± 6 ml/100 g/min in DMSO-treated mdr1a(–/–) mice, p > 0.05].
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Similar to the results obtained from the single-dose rifampin treatment experiment, coperfusion of rifampin was much less potent in inhibiting of P-gp-mediated quinidine efflux compared with verapamil efflux. The degree of inhibition of P-gp-mediated efflux of quinidine by coperfusion of rifampin at concentrations of 500 and 1000 µM was approximately 30 and 40%, respectively (Fig. 5).
Influence of Verapamil Coperfusion on Brain Uptake of Quinidine.
Coperfusion of verapamil was able to inhibit P-gp-mediated quinidine efflux in
the BBB (Fig. 6). However, the
degree of inhibition was not significantly different among different verapamil
concentrations (p > 0.05). The pooled maximum inhibition of
P-gp-mediated quinidine efflux by coperfusion of verapamil was 63%.
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Discussion |
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TopAbstractMaterials and MethodsResultsDiscussionReferences |
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Rifampin was selected to induce P-gp in mouse brain because it is a potent
inducer of P-gp both in human duodenal biopsies (3.5-fold)
(Greiner et al., 1999) and in
human colon carcinoma cell lines (Schuetz
et al., 1996). Morphine has been shown to increase P-gp content
about 2-fold in rat brain after a 5-day treatment
(Aquilante et al., 2000).
However, in the present studies both agents induced P-gp expression in mouse
brain to only a modest extent (40 and 50% increase with morphine and
rifampin treatment, respectively; the changes associated with morphine
treatment did not achieve statistical significance). This discrepancy may be
due to species differences and/or tissue specificities in xenobiotic-mediated
induction of P-gp expression in the brain. Such differences are not unusual.
For instance, rifampin is an efficacious inducer of cytochrome P450 3A (CYP3A)
in humans but not in rodents (LeCluyse,
2001). Similarly, dexamethasone increased P-gp expression more
than 4.5- and 2-fold in rat liver and lung, respectively, whereas it decreased
P-gp expression 40% in kidney (Demeule et
al., 1999). Further studies are required to identify more
effective inducers of brain P-gp to study the dynamics of P-gp induction in
the BBB.
The results of functional tests after P-gp induction by rifampin were
unanticipated. There was a significant increase in verapamil brain uptake,
rather than the anticipated decrease in verapamil CLup, after
pretreatment with rifampin (Fig.
2). This observation suggests that inhibition of P-gp by rifampin
masks whatever increase in P-gp-mediated transport might occur secondary to
rifampin pretreatment. It is possible that rifampin binds tightly to the brain
capillaries due to its high lipophilicity, thus evidencing a prolonged
residence time in the BBB or the brain parenchyma. Several early studies have
shown that rifampin can inhibit P-gp activity in vitro
(Fardel et al., 1995;
Furusawa et al., 1997).
Functional tests with an acute dose of rifampin indeed demonstrated a
significant inhibitory effect on BBB P-gp
(Fig. 2). Therefore, induced
P-gp activity by multiple doses of rifampin might actually be masked by an
inhibitory effect of rifampin itself.
Further assessment of the dynamics of P-gp inhibition by acute rifampin was
conducted using verapamil and quinidine as model compounds because of their
moderate to high P-gp effect in situ
(Dagenais et al., 2001). These
experiments revealed a dose-dependent inhibition of P-gp-mediated efflux,
although the degree of rifampin-associated inhibition differed between the two
substrates (Fig. 3). The
maximum inhibition of P-gp-mediated verapamil efflux was 55% at a
rifampin dose of 150 mg/kg, whereas there was only a maximum inhibition of
12% for P-gp-mediated quinidine efflux. These results are consistent with
the fact that quinidine has a higher P-gp effect than verapamil at the murine
BBB. The brain uptake of both verapamil and quinidine was unaffected by a 100
mg/kg i.p. dose of rifampin in mdr1a(–/–) mice compared
with the controls, suggesting that transporters other than mdr1a
isoform encoded P-gp were not involved.
Pretreatment with rifampin was only able to partially abolish P-gp activity
in the BBB in situ. This incomplete inhibition may be due to an inability to
achieve sufficiently high rifampin concentrations in the BBB after systemic
administration because of dose-limiting toxicity. Alternatively, rifampin may
not be able to block completely P-gp activity in the BBB. The latter
hypothesis was not supported because rifampin was able to inhibit almost
completely P-gp activity in the BBB during coperfusion with verapamil
(Fig. 5). Verapamil
CLup in mdr1a(+/+) mice coperfused with 500 µM rifampin
was not statistically different from that in mdr1a gene-deficient
mice (p > 0.05). More importantly, the degree of P-gp inhibition
by pretreatment with rifampin was in good agreement with the results from the
coperfusion study. When the data are plotted on the same set of axes
(Fig. 7), the
concentration-dependent change in verapamil efflux transport is nearly
identical between the two experiments, suggesting that the method of treatment
was not important (i.e., derived metabolites do not contribute to the
inhibitory effect) and that the concentration of the inhibitor dictates the
degree of inhibition. In addition, total concentrations of rifampin in the
cerebral vasculature (i.e., unbound rifampin in the coperfusion study, in
which the perfusate was protein-free; bound plus unbound rifampin after in
vivo pretreatment) seem to serve as the driving force for P-gp inhibition. In
contrast, rifampin seemed to be unable to inhibit completely P-gp-mediated
quinidine efflux even at very high concentrations (i.e., 1000 µM in the
perfusate; Fig. 5). The maximum
inhibition based on the data from both pretreatment and coperfusion of
rifampin studies was 42% (Fig.
8), which was comparable with the ability of verapamil to inhibit
quinidine transport (63% inhibition;
Fig. 6). These results were
intriguing. As evidenced in the present study, rifampin was able to completely
inhibit P-gp-mediated verapamil efflux in the BBB. In addition, quinidine has
been shown to be able to restore verapamil brain uptake in mdr1a(+/+)
mice to the level of mdr1a(–/–) mice (C. Dagenais,
personal communication). However, both rifampin and verapamil were only able
to partially block P-gp-mediated quinidine efflux in the BBB. It has been
suggested that there are multiple binding sites on the P-gp
(Shapiro et al., 1999;
Martin et al., 2000). One
possible explanation for the current observation is that verapamil and
rifampin may bind to the same site(s) on P-gp, whereas quinidine may interact
with other site(s) in addition to the verapamil/rifampin site. This hypothesis
was further supported by observations reported by Wang et al.
(2000). They have shown that
the P-gp substrate H33342
[GenBank]
interact with quinidine in a noncompetitive manner,
whereas it interacts with verapamil in a mixed mode of inhibition.
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In conclusion, the present studies have shown that P-gp function in the BBB can be modulated by rifampin in a dose- and concentration-dependent manner. The results also suggest that perturbations in the disposition of P-gp substrates in the brain may be predicted based on the extent of P-gp modulation (e.g., inhibition or induction).
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Footnotes |
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ABBREVIATIONS: P-gp, P-glycoprotein; MDR, multidrug resistance; BBB, blood-brain barrier; DMSO, dimethyl sulfoxide; CLup, uptake clearance; HPLC, high-performance liquid chromatography; PSC833, valspodar; H33342 [GenBank] , 2-(4-ethoxyphenyl)-5-(4-methyl-1-piperazinyl)-2,5-bi-1H-benzimidazole trihydrochloride.
Address correspondence to: Dr. Gary M. Pollack, Division of Drug Delivery and Disposition, School of Pharmacy, University of North Carolina at Chapel Hill, Chapel Hill, NC 27599. E-mail: gary_pollack{at}unc.edu
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References |
|---|
|
TopAbstractMaterials and MethodsResultsDiscussionReferences |
|---|
Ambudkar SV, Dey S, Hrycyna CA, Ramachandra M, Pastan I, and Gottesman MM (1999) Biochemical, cellular and pharmacological aspects of the multidrug transporter. Annu Rev Pharmacol Toxicol 39: 361–398.[CrossRef][Medline]
Aquilante CL, Letrent SP, Pollack GM, and Brouwer KL (2000) Increased brain P-glycoprotein in morphine tolerant rats. Life Sci 66: PL47–PL51.[Medline]
Bergwerk AJ, Shi X, Ford AC, Kanai N, Jacquemin E, Burk RD, Bai S, Novikoff PM, Stieger B, Meier PJ, et al. (1996) Immunologic distribution of an organic anion transport protein in rat liver and kidney. Am J Physiol 271: G231–G238.
Chen C and Pollack GM (1998) Altered disposition and
antinociception of [D-penicillamine2,5]enkephalin in
mdr1a-gene-deficient mice. J Pharmacol Exp
Ther 287:
545–552.
Cordon-Cardo C, O'Brien JP, Casals D, Rittman-Grauer L, Biedler JL,
Melamed MR, and Bertino JR (1989) Multidrug-resistance gene
(P-glycoprotein) is expressed by endothelial cells at blood-brain barrier
sites. Proc Natl Acad Sci USA
86:
695–698.
Dagenais C, Rousselle C, Pollack GM, and Scherrmann JM (2000) Development of an in situ mouse brain perfusion model and its application to mdr1a P-glycoprotein-deficient mice. J Cereb Blood Flow Metab 20: 381–386.[Medline]
Dagenais C, Zong J, Ducharme J, and Pollack GM (2001) Effect of mdr1a P-glycoprotein gene disruption, gender and substrate concentration on brain uptake of selected compounds. Pharm Res (NY) 18: 957–963.[CrossRef][Medline]
Demeule M, Jodoin J, Beaulieu E, Brossard M, and Beliveau R (1999) Dexamethasone modulation of multidrug transporters in normal tissues. FEBS Lett 442: 208–214.[CrossRef][Medline]
Fardel O, Lecureur V, Loyer P, and Guillouzo A (1995) Rifampicin enhances anti-cancer drug accumulation and activity in multidrug-resistant cells. Biochem Pharmcol 49: 1255–1260.[CrossRef][Medline]
Fromm MF, Eckhardt K, Li S, Schanzle G, Hofmann U, Mikus G, and Eichelbaum M (1997) Loss of analgesic effect of morphine due to coadministration of rifampin. Pain 72: 261–267.[CrossRef][Medline]
Furusawa S, Nakano S, Wu J, Sasaki K, Takayanagi M, and Takayanagi Y (1997) Potentiation of pirarubucin activity in multidrug resistant cells by rifampicin. Biol Pharm Bull 20: 1303–1306.[Medline]
Gottesman MM and Pastan I (1993) Biochemistry of multidrug resistance mediated by the multidrug transporter. Annu Rev Biochem 62: 385–427.[CrossRef][Medline]
Greiner B, Eichelbaum M, Fritz P, Kreichgauer HP, von Richter O, Zundler J, and Kroemer HK (1999) The role of intestinal P-glycoprotein in the interaction of digoxin and rifampin. J Clin Investig 104: 147–153.[Medline]
Hsu SI, Lothenstein L, and Horwitz SB (1989)
Differential overexpression of three mdr gene family members in
multidrug resistant J774.2 mouse cells. Evidence that distinct P-glycoprotein
precursors are encoded by unique mdr genes. J Biol
Chem 264:
12053–12062.
Hyafil F, Vergely C, Du Vignaud P, and Grand-Perret T
(1993) In vitro and in vivo reversal of
multidrug resistance by GF120918, an acridonecarboxamide derivative.
Cancer Res 53:
4595–4602.
Juliano RL and Ling V (1976) A surface glycoprotein modulating drug permeability in Chinese hamster ovary cell mutants. Biochim Biophys Acta 455: 152–162.[Medline]
LeCluyse EL (2001) Pregnane X receptor: molecular basis for species differences in CYP3A induction by xenobiotics. Chem Biol Interact 134: 283–289.[CrossRef][Medline]
Lee CG, Gottesman MM, Cardarelli CO, Ramachandra M, Jeang KT, Ambudkar SV, Pastan I, and Dey S (1998) HIV-1 protease inhibitors are substrates for MDR1 multidrug transporter. Biochemistry 37: 3594–3601.[CrossRef][Medline]
Lemaire M, Bruelisauer A, Guntz P, and Sato H (1996) Dose-dependent brain penetration of SDZ PSC 833, a novel multidrug resistance-reversing cyclosporin, in rats. Cancer Chemother Pharmacol 38: 481–486.[CrossRef][Medline]
Leveille-Webster CR and Arias IM (1995) The biology of the P-glycoproteins. J Membr Biol 143: 89–102.[Medline]
Lowry OH, Rosebough NJ, Farr AL, and Randal RJ (1951)
Protein measurement with the folin phenol reagent. J Biol
Chem 193:
265–275.
Martin C, Berridge G, Higgins C, Mistry P, Charlton P, and
Callaghan R (2000) Communication between multiple drug binding
sites on P-glycoprotein. Mol Pharmacol
58:
624–632.
Prince C, Miller DW, Stemmer PM, Strong ML, Ueda CT, and Elmoquist WF (1996) The effect of chronic oral dosing cyclosporine A on the expression of P-glycoprotein in the rat. Pharm Res (NY) 13: S456.
Ruetz S and Gros P (1994) Phosphotidylcholine translocase: a physiological role for the mdr2 gene. Cell 77: 1071–1081.[CrossRef][Medline]
Schinkel AH (1997) The physiological function of drug-transporting P-glycoproteins. Semin Cancer Biol 8: 161–170.[CrossRef][Medline]
Schuetz EG, Beck WT, and Schuetz JD (1996) Modulators and substrates of P-lycoprotien and cytochrome P4503A coordinately up-regulate these proteins in human colon carcinoma cells. Mol Pharmacol 49: 311–318.[Abstract]
Shapiro AB, Fox K, Lam P, and Ling V (1999) Stimulation of P-glycoprotein-mediated drug transport by prazosin and progesterone. Evidence for a third drug-binding site. Eur J Biochem 259: 841–850.[Medline]
Smit JJ, Schinkel AH, Oude Elferink RP, Groen AK, Wagenaar E, van Deemter L, Mol CA, Ottenhoff R, van der Lugt NM, and van Roon MA (1993) Homozygous disruption of the murine mdr2 P-glycoprotein gene leads to a complete absence of phospholipid from bile and to liver disease. Cell 75: 451–462.[CrossRef][Medline]
Smith QR (1996) Brain perfusion systems for studies of drug uptake and metabolism in the central nervous system, in Models for Assessing Drug Absorption and Metabolism (Borchardt RT, Smith PL, and Wilson G eds) pp 285–307, Plenum Press, New York.
Thiebaut F, Tsuruo T, Hamada H, Gottesman MM, Pastan I, and
Willingham MC (1987) Cellular localization of the
multidrug-resistance gene product P-glycoprotein in normal human tissues.
Proc Natl Acad Sci USA
84:
7735–7738.
Wang EJ, Casciano CN, Clement RP, and Johnson WW (2000) Two transport binding sites of P-glycoprotein are unequal yet contingent: initial rate kinetic analysis by ATP hydrolysis demonstrates intersite dependence. Biochim Biophys Acta 1481: 63–74.[CrossRef][Medline]
Zong J and Pollack GM (2000) Morphine antinociception
is enhanced in mdr1a Gene-deficient mice. Pharm Res
(NY) 17:
749–753.[CrossRef][Medline]
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