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Vol. 283, Issue 3, 1552-1562, 1997
Departments of Pharmaceutics (M.F.P., M.K., J.M.F., D.D.S., K.E.T.), Medicinal Chemistry (K.L.K.) and Surgery (C.L.M., J.D.P.), University of Washington, Seattle, Washington
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Abstract |
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Abstract
Introduction
Methods
Results
Discussion
References
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Cytochrome P450 3A (CYP3A) metabolizes a diverse array of clinically
important drugs. For some of these (e.g., cyclosporine, verapamil, midazolam), CYP3A in the intestinal mucosa contributes to
their extensive and variable first-pass extraction. To further characterize this phenomenon, we measured CYP3A content and catalytic activity toward the probe substrate midazolam in mucosa isolated from
duodenal, jejunal and ileal sections of 20 human donor intestines. For
comparison, the same measurements were performed for 20 human donor
livers, eight of which were obtained from the same donors as eight of
the intestines. Excellent correlations existed between homogenate and
microsomal CYP3A content for the three intestinal regions. Median
microsomal CYP3A content was greatest in the duodenum and lowest in the
ileum (31 vs. 17 pmol/mg of protein). With respect to
midazolam 1
-hydroxylation kinetics, the median
Km for each intestinal region was similar to the
median hepatic Km, ~4 µM. In contrast, the
median Vmax decreased from liver to duodenum to
jejunum to ileum (850 vs. 644 vs. 426 vs. 68 pmol/min/mg). Intrinsic clearance
(Vmax/Km) followed a
similar trend for the intestinal regions; median duodenal intrinsic
clearance was comparable to hepatic intrinsic clearance (157 and 200 µl/min/mg, respectively). Vmax correlated with
CYP3A content for all tissues except the ileum. Duodenal and jejunal
Vmax and CYP3A content varied by >30-fold among
donors. Microsomes prepared from every other 1-foot section of six
intestines were also analyzed for CYP3A as well as for two coenzymes.
In general, CYP3A activity, CYP3A content and CYP reductase activity
rose slightly from duodenum to middle jejunum and then declined to
distal jejunum and ileum. Cytochrome b5 content and cytochrome b5 reductase activity varied
little throughout the intestinal tract. Regional intrinsic midazolam
1-hydroxylation clearance was greatest for the jejunum, followed by
the duodenum and ileum (144, 50 and 19 ml/min, respectively).
Collectively, these results demonstrate that the upper small intestine
serves as the major site for intestinal CYP3A-mediated first-pass
metabolism and provides a rationale for interindividual differences in
oral bioavailability for some CYP3A substrates.
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Introduction |
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Abstract
Introduction
Methods
Results
Discussion
References
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Human
cytochrome P450 3A isoforms (CYP3A) metabolize a number of widely
prescribed, structurally diverse drugs that belong to a variety of
therapeutic classes (Guengerich, 1995
; Wrighton and Stevens, 1992).
CYP3A4 and CYP3A5 are the major isoforms expressed in adults. Although
found in many tissues throughout the body, their relative levels of
expression are greatest in the liver and villus epithelium of the small
intestine. On average, CYP3A composes 25% to 30% of total hepatic
cytochromes P450 (Shimada et al., 1994; Wrighton and
Stevens, 1992) and an even larger percentage of total small intestinal
cytochromes P450 (De Waziers et al., 1990; Watkins et
al., 1987). In addition, CYP3A content in both organs is highly
variable among individuals. Lown et al. (1994) found CYP3A4
protein to vary >11-fold in S9 fractions prepared from 20 human
duodenal biopsies, and Shimada et al. (1994) found a similar
variability in liver microsomes prepared from 60 human samples.
Due to the anatomic arrangement of the small intestine and liver, drugs
may encounter sequential, CYP3A-mediated first-pass metabolism when
taken orally (Thummel et al., 1997). Historically, the liver
was considered the major site of CYP3A-dependent first-pass metabolic
extraction. Recent in vitro and in vivo studies,
however, suggest that mucosal villi of the small intestine can be of
equal or greater importance for some drugs such as cyclosporine (Gomez et al., 1995; Hebert et al., 1992; Kolars
et al., 1991; Webber et al., 1992) and verapamil
(Fromm et al., 1996). We also conducted a series of human
studies that indicate extensive intestinal first-pass metabolism of the
sedative/hypnotic agent MDZ. MDZ is eliminated entirely (>97%) by
oxidative biotransformation reactions catalyzed by the CYP3A subfamily
(Fabre et al., 1988; Gorski et al., 1994; Kronbach et al., 1989). A pharmacokinetic analysis of
intravenous and oral MDZ disposition in healthy volunteers (Thummel
et al., 1996) suggested that the low oral bioavailability
observed for this drug (mean, 30 ± 10%) was the result of
comparable extraction ratios for the liver (mean, 44 ± 14%) and
intestine (mean, 43 ± 24%). Direct measurements of first-pass
MDZ extraction during the anhepatic phase of liver transplant
operations confirmed an identical mean gut wall extraction fraction
(43 ± 18%) (Paine et al., 1996). Both in
vivo MDZ studies revealed large interindividual differences in
hepatic and intestinal extraction ratios. Hepatic extraction ranged
from 22% to 76%, whereas intestinal extraction ranged from ~0% to
77% (healthy volunteer study) and from 14% to 59% (anhepatic study).
These interindividual variations are consistent with variably expressed
CYP3A content and associated in vitro MDZ 1-hydroxylation
activity measured in human liver microsomes (Kronbach et
al., 1989) and in S9 fractions prepared from human duodenal
biopsies (Lown et al., 1994).
The intravenous formulation of MDZ (Versed), administered orally or
directly into the duodenum, is absorbed rapidly from the most proximal
region of the small intestine. Other CYP3A substrates that have slow
dissolution or administered in sustained-release formulations are
absorbed throughout the small intestinal tract. Because mucosal CYP3A4
content is reportedly lower in jejunum and ileum compared with duodenum
(De Waziers et al., 1990), first-pass intestinal metabolic
extraction may depend on the absorption characteristics of the drug
formulation; that is, first-pass intestinal metabolism may be reduced
when drug is absorbed at more distal sites of the small intestine.
However, very little is known about the extent of interindividual
variability in CYP3A expression in epithelium distal to the duodenum as
well as the relative catalytic capacities of duodenal, jejunal and
ileal CYP3A.
We characterized CYP3A protein content and catalytic activity, as well
as two CYP coenzymes (NADPH-dependent cytochrome P450 reductase and
cytochrome b5), along the entire length of six
different human donor small intestines. In addition, we determined the
relative metabolic capacity (MDZ intrinsic clearance) of the three
regions (duodenum, jejunum and ileum) in 15 donor small intestines. For comparison, parallel analyses were performed with 20 human livers. Based on these in vitro results, we estimated whole-organ
intrinsic clearances using a conventional flow model (Pond and Tozer,
1984; Wilkinson, 1987) and considered their correlation to gut and
liver extraction of MDZ in vivo.
| |
Methods |
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Abstract
Introduction
Methods
Results
Discussion
References
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Chemicals.
MDZ, 1-OH MDZ and 4-OH MDZ were kindly provided
by Drs. William Garland and Bruce Mico (Roche Laboratories, Nutley,
NJ). Cytochrome c (horse heart type VI), NADPH (reduced
form, tetrasodium salt), NADH, EDTA, PMSF and anti-rabbit IgG alkaline
phosphatase conjugate were purchased from Sigma Chemical (St. Louis,
MO). N-Methyl-N-(t-butyl-dimethylsilyl)trifluoroacetamide
was purchased from Pierce Chemical (Rockford, IL). Acetonitrile and
ethyl acetate were purchased from Fisher Scientific (Santa Clara, CA).
SDS-PAGE reagents (SDS, acrylamide, ammonium persulfate, TEMED) were
purchased from BioRad (Hercules, CA). Nitrocellulose was purchased from Schleicher & Schuell (Keene, NH). BCIP-NBT was purchased from Kirkegaard and Perry (Gaithersburg, MD). All other chemicals were of
reagent grade or better.
Organ procurement.
The collection and use of human donor
tissue for research were approved by the University of Washington Human
Subjects Review Board. During procurement, the liver and small
intestine were dissected in preparation for removal and then perfused
in situ with cold (4°C) University of Wisconsin solution
(Viaspan). The organs were kept cold with topical iced saline until
removal from the abdominal cavity. After retrieval and transport of
each intestine (in "iced saline") to our laboratory, the organ was
cut into 1-foot sections, flushed with ~60 ml cold saline and
weighed. Sections of mucosa were exposed by a longitudinal cut and
carefully scraped free from the remainder of the gut tissue using a
glass slide. Mucosal scrapings from each section were then placed
separately into 45 ml conical polypropylene tubes, weighed, immediately
frozen in liquid nitrogen and stored at 
70°C. All processing of
tissue was performed on a bed of ice. Full-length small intestines from a total of 20 donors were used for study.
The time elapsed between vascular cross-clamp (start of cold ischemia)
and the freezing of all mucosal scrapings was usually <3 hr. Two
intestines were obtained from out-of-state donors (Alaska and Oregon).
Transit and processing time of these organs were <5 hr. Procured
livers were kept on ice for a more variable period of time, 12 to 24 hr, before processing. After transfer to our laboratory, the organs were cut into ~10 g pieces and snap-frozen in liquid nitrogen. Tissue
from a total of 20 livers was used for study. Six exhibited fatty
infiltration in >25% of parenchymal cells. Three livers were obtained
from out-of-state donors (Idaho, Montana and Alaska), and eight livers
were from the same donors as 8 of the 20 intestines. There were an
equal number of male and female intestine donors, but 12 female and 8 male liver donors. The age range for both liver and intestine donors
was 10 to 70 years, and nearly all were Caucasian.
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Preparation of hepatic and intestinal microsomes.
Hepatic
microsomes were prepared from 20 livers as described previously
(Thummel et al., 1993), except that 0.25 M sucrose containing 1 mM EDTA was used as the storage solution. Intestinal microsomes were prepared from every other 1-foot section of six whole
small intestines and from a 1-foot section of each of the three regions
(duodenum, jejunum and ileum) of an additional 14 whole small
intestines as described previously (Thummel et al., 1996)
with some modifications. Briefly, homogenizing buffer (10 mM potassium
phosphate, pH 7.4, containing 0.25 M sucrose, 1 mM EDTA and 0.1 mM
PMSF) was added directly to the frozen conical tubes containing the
mucosal scrapings (5-fold v/v dilution). After the tissue was thawed,
the mixture was transferred to and homogenized in a 55-ml glass Wheaton
tube using a motor-driven Teflon-tipped pestle (8-10 strokes). The
total volume of homogenate was recorded, and two 1-ml aliquots were
saved. Homogenate was transferred to 30-ml centrifuge tubes, which were
spun at 600 × g for 5 min and then at 11,000 × g for 15 min. The resulting supernatant was filtered through
sterile gauze into 60-ml centrifuge tubes, which were spun at
110,000 × g for 70 min. After saving the supernatant
for unrelated studies, the remaining pellet was resuspended in wash
buffer (10 mM potassium phosphate, pH 7.4, containing 1 mM EDTA and 0.1 mM PMSF) and centrifuged again at 110,000 × g for 70 min. The washed pellet was resuspended in storage solution (0.25 M
sucrose, pH 7.4, containing 1 mM EDTA and 0.1 mM PMSF) to a final
protein concentration of 10 to 30 mg/ml. Aliquots of the final
microsomal suspension (~0.25 ml) were stored at 70°C. Protein
concentrations were determined according to the method of Lowry
et al. (1951) using bovine serum albumin as the reference standard.
Spectrophotometric assays.
Total cytochrome P450 and
cytochrome b5 concentrations in hepatic and
intestinal microsomes were measured according to the method of Omura
and Sato (1964) using extinction coefficients of 91 and 185 mM
1 cm1, respectively. Microsomal
cytochrome P450 reductase and cytochrome b5
reductase activities were measured by determining the rates of NADPH-
and NADH-dependent cytochrome c reduction, respectively, as
described previously (Kurzban and Strobel, 1986). Briefly, 100 µg of
microsomal protein, cytochrome c and either NADPH or NADH
were mixed with potassium phosphate buffer (0.3 M, pH 7.7) to a final
1-ml volume in a cuvette. The final concentrations of cytochrome
c, NADPH and NADH were 40 µM, 1 mM and 0.64 mM, respectively. Immediately after the addition of NADPH or NADH, the
change in absorbance (550-538 nm) was measured every 3 sec over 60 sec
at 25°C. The rates of cytochrome c reduction were calculated using an extinction coefficient of 21 mM1
cm1 (Van Gelder and Slater, 1962).
Western blot analysis of CYP3A4 and CYP3A5.
Both homogenate
and microsomes were analyzed for these two proteins. Intestinal
microsomes, intestinal homogenate and hepatic microsomes were diluted
in sample buffer (60 mM Tris · HCl, 25% glycerol, 0.2% Emulgen
911, pH 7.4) to final concentrations of 20 to 50, 50 and 5 µg/20
µl, respectively. After boiling each sample for 2 min, 20 µl was
loaded onto 0.1% SDS-9% acrylamide gels, and the proteins were
separated as described previously (Favreau et al., 1987).
Purified CYP3A4 standards (Kharasch and Thummel, 1993) were also
prepared and run in parallel with the microsomal or homogenate samples.
At the end of the run (~3.5 hr), the proteins were
electrophoretically transferred to nitrocellulose; the sheet was rinsed
twice with PBS and stored in blocking buffer (2% nonfat dry milk and
2% Triton X-100 in PBS) overnight. The following morning, the
nitrocellulose sheets were incubated with a selective rabbit polyclonal
anti-CYP3A4 IgG (Kharasch and Thummel, 1993) at a final concentration
of 1 µg/ml in blocking buffer for 2 hr at room temperature. The
sheets were washed twice with blocking buffer and then incubated with
the secondary antibody, anti-rabbit IgG alkaline phosphatase conjugate
(1:1000), for 2 hr. The sheets were washed twice with blocking buffer,
twice with PBS and twice with 0.1 M Tris buffer (pH 7.4). The proteins
of interest were visualized with the addition of BCIP-NBT according to
the manufacturer's instructions. A protein band that comigrated with
the CYP3A4 standard was detected in all samples. A second, slightly
higher-molecular-weight protein band was also detected in 20% of
livers and intestines; this was presumed to be CYP3A5. All blots were
scanned (Howtek Scanmaster 3+) and quantified for CYP3A4 and CYP3A5 by
densitometry using the software programs Visage and Whole Band Analysis
(v4.6M and v2.4, respectively; Millipore BioImage Products, Ann Arbor, MI). Purified CYP3A4 was used as the reference standard.
Hepatic and intestinal microsomal incubations.
An internal
standard mixture containing 15N3-labeled MDZ
metabolites (i.e., 1-OH MDZ and 4-OH MDZ) was prepared by
incubating 6 nmol of cytochrome P450 (using HL-122 microsomes) with 100 µg of 15N3-MDZ and 12 mg of NADPH (final
concentration, ~1.5 mM) in potassium phosphate buffer (0.1 M, pH 7.4, in a final volume of 8 ml) at 37°C. After 10 min, the reaction was
stopped by the addition of 8 ml of Na2CO3 (0.1 M, pH 12). The compounds were extracted twice with 20 ml of ethyl
acetate, and the solvent was evaporated to dryness under a stream of
nitrogen. The remaining solid was then reconstituted in 20 ml of
methanol, split into two 10-ml aliquots and stored at 20°C.
-OH MDZ formation rate. Duplicate
incubation mixtures containing 100 to 200 µg of microsomal protein
(metabolite formation was found to be linear with microsomal protein up
to 500 µg of protein) and 100 µl of 80 µM MDZ in potassium
phosphate buffer (total volume of 0.9 ml) were preincubated at 37°C
for 5 min. The reaction was initiated by the addition of 100 µl of 10 mM NADPH; final concentrations of MDZ and NADPH were 8 µM and 1 mM,
respectively. The reaction was terminated after 4 min by the addition
of 1 ml of Na2CO3 (final pH ~11). Alkalinized
samples were spiked with 100 µl of a 1:5 dilution of the internal
standard mixture (in distilled, deionized water), which represented
~50 and ~10 ng of 15N3-labeled 1-OH MDZ
and 4-OH MDZ, respectively. The metabolites were extracted with 5 ml of
ethyl acetate, the solvent was removed under nitrogen and the
concentrated extracts were dissolved in 100 µl of derivatizing
reagent [10%
N-methyl-N-(t-butyl-dimethylsilyl)trifluoroacetamide in
acetonitrile]. The samples were then transferred to autoinjector vials
and sealed before being heated at 80°C for 2 hr before analysis.
Michaelis-Menten parameters Vmax and
Km for 1-OH MDZ formation were determined in
microsomes prepared from all livers and from the three regions of 15 intestines. Incubation conditions were the same as described earlier
except that eight MDZ concentrations were used (0, 0.25, 0.5, 1, 2, 4 and 8 µM) and microsomal protein ranged from 20 to 50 µg and from
50 to 300 µg for liver and intestine, respectively. Initial estimates
of Vmax and Km were
determined by applying the Eadie-Hofstee transformation for a unienzyme
system to the product formation rate data. Final parameter estimates were obtained by nonlinear least-squares regression of unweighted data
using PCNONLIN (v4.2, SCI Software, Lexington, KY). The unbound intrinsic clearance, Clin,mic, was calculated by dividing
Vmax by Km.
Because CYP3A5-containing livers were found to have higher product
ratios (1-OH MDZ/4-OH MDZ) than those without CYP3A5 (Gorski et
al., 1994), the catalytic activities of three CYP3A5-containing jejunal samples were further examined by measuring the same product ratios and comparing them with three intestines that did not contain CYP3A5. Similar incubations were also carried out with six livers. Incubation conditions were again the same as those described earlier except that four MDZ concentrations were used: 0.25, 1, 4 and 8 µM.
Incubates were analyzed for 4-OH MDZ and/or 1-OH MDZ by selective ion
gas chromatography-negative chemical ionization mass spectrometry
(GC/NCI-MS) as previously described (Paine et al., 1996)
except that molecular ions with m/z 455 and 460 (corresponding to the unlabeled and
15N3-labeled 37Cl isotope of 1-OH
MDZ, respectively) and base peak fragment ions
([M-tBu(CH3)2SiOH])
with m/z 323 and 328 (corresponding to the unlabeled and
15N3-labeled 37Cl isotope of 4-OH
MDZ, respectively) were monitored. The GC column retention time for
4-OH MDZ was slightly shorter than 1-OH MDZ (12.7 vs. 14.0 min). The two metabolites were quantified by comparing peak area ratios
with standard curves prepared by the addition of known amounts of 4-OH
MDZ (0.3-30 pmol) and/or 1-OH MDZ (1.5-300 pmol) and 100 µl of
internal standard to phosphate buffer. The interassay coefficient of
variation in the slopes from the standard curves for 4-OH MDZ and 1-OH
MDZ were 8.1% and 5.2%, respectively.
Determination of a correction factor for homogenate protein. With Western blot analysis, we compared the slope obtained from a standard curve using purified CYP3A4 only (i.e., 0, 0.5, 1 and 2 pmol) with that using purified CYP3A4 spiked into 50 µg of jejunal homogenate protein (i.e., 50 µg of protein plus 0.5, 1 or 2 pmol). The slope (change in IOD/change in pmol CYP3A4 added) from the CYP3A4-only curve was higher than that obtained from the standard addition curve. Therefore, to correct for this "matrix effect," five additional jejunal homogenates were randomly chosen and subjected to Western blot analysis as described previously. Again, the slopes from the purified CYP3A4-only standard curves were consistently higher than those from the standard addition curves. The correction factor (slope without homogenate/slope with homogenate) for the six homogenates averaged 1.26 ± 0.29. The median was 1.23 and was used to correct for the median amount of homogenate CYP3A determined from earlier blots. Only corrected medians are reported. We did not find a noticeable matrix effect from microsomal protein and thus did not apply a correction factor to median amounts of microsomal CYP3A.
Calculation of total CYP3A recovery and organ intrinsic
clearance.
Based on a previous study of the physical
characteristics (i.e., weight and length) of human small
intestine (Snyder et al., 1975), we assigned the first
1-foot section as the duodenum, sections 2 to 9 as the jejunum and the
remaining sections as the ileum. The total mucosal scrapings mass per
gram of intestinal tissue was recorded for each section of seven
organs, and regional (duodenal, jejunum, ileal) wet weights were
determined accordingly. Total CYP3A in each of the three regions was
then calculated using the following equation:
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(1) |
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(2) |
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-OH MDZ formation clearance for each of the three regions of human
small intestine. For comparison, total intrinsic clearance for the
liver was calculated using a liver weight of 1500 g (Snyder
et al., 1975), the median hepatic Clin,mic, and
assuming an average microsomal protein recovery of 52.5 mg/g liver
(Iwatsubo et al., 1997). This recovery value was obtained from hepatocyte cultures, which we believe is more accurate than that
obtained from recovered microsomal protein.
To determine an in vitro-in vivo "scaling factor" for
each intestinal region (i.e., a number that could be used to
scale microsomal intrinsic clearance for any substrate to total
regional clearance), we estimated the total amount of microsomal
protein in each region for the seven intestines from which we had
complete data sets. Assuming that microsomal CYP3A content from a
1-foot section was representative of the entire intestinal region, the
scaling factor for each region was calculated as follows:
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(3) |
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(4) |
Statistical analysis.
All statistical analyses were
performed using Sigmastat for Windows (v1.0, Jandel Corp., San Rafael,
CA). Because several data sets failed the homogeneity-of-variance and
normality tests (Levene Median and Kolmogorov-Smirnov tests,
respectively), nonparametric methods were used for the majority of
analyses. Average values were reported for comparisons of 1-OH MDZ
with 4-OH MDZ ratios because the sample sizes were <5. Spearman
correlation coefficients (rs) were considered
significant if the P-value was <0.05. One-way ANOVA on ranks
(Kruskal-Wallis) was used to determine whether a difference existed in
the various kinetic parameter estimates and CYP3A contents among the
liver, duodenum, jejunum and ileum (and ignoring that each set of three
intestinal regions came from the same donor and that eight livers and
intestines were matched; this resulted in a less powerful but more
conservative test). For the three intestines from which we could not
obtain reliable parameter estimates for one or two regions (due to low
CYP3A activity), median regional Km values were
assumed along with Vmax and Clin,mic values that were ranked lower than the corresponding regional minimum
Vmax and Clin,mic. Likewise, for
intestinal regions for which the protein band was too faint to be
detected by the densitometer, a ranking lower than the regional minimum
was assumed. Further, if ANOVA revealed a significant difference
(P < 0.05), then either the Student-Newman-Keuls test (for equal
sample sizes) or Dunn's test (for unequal samples sizes) was used to
determine which group medians differed from the others. To compare the
three intestinal regions, taking into account that each set of three
came from the same donor, three pairwise Wilcoxon signed-rank tests
were used along with a Bonferroni-corrected level of significance, 0.017 (i.e., 0.05/3).
| |
Results |
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Abstract
Introduction
Methods
Results
Discussion
References
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Total CYP, cytochrome b5 and CYP3A contents. Western blot analysis of microsomes from 20 livers and small intestines showed the presence of CYP3A4 protein in every organ and CYP3A5 protein in four livers and four intestines. A representative blot illustrating the continuous expression of CYP3A5 along the entire length of small intestine is shown in figure 1. Concordant hepatic-intestinal expression of CYP3A4 and CYP3A5 was observed in seven of the eight matched organs (table 1). Six of the seven concordant organs expressed CYP3A4 only, whereas one pair expressed both CYP3A4 and CYP3A5. For the single discordant pair (HL-147/HI-26), both proteins were detected in the liver, but only CYP3A4 was detected in the intestine. Also, although a modest CYP3A4 protein band was detected in the jejunum and ileum of HI-26, no band was detected (by the densitometer) for the duodenum. The CYP3A5-to-CYP3A4 IOD ratio in CYP3A5-positive organs was less than unity in all except one liver and two ileal sections of its intestinal mate. This interpretation may be biased because the detection antibody was raised against purified CYP3A4 protein.
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MDZ 1-hydroxylation kinetics.
Fifteen intestines were
examined for regional (duodenal, jejunal and ileal) MDZ
1-hydroxylation kinetics. However, in some regions of three
intestines, the amount of product formed was below the limit of
quantification at low substrate concentrations and, in some cases, at
all substrate concentrations. Thus, we could not obtain reliable
kinetic parameter estimates in these cases. Representative
Eadie-Hofstee plots of 1-OH MDZ formation kinetics for each of the
three intestinal regions of one small intestine are shown in figure
2. All 20 liver microsomal samples produced amounts of product that were readily quantifiable (at all
substrate concentrations), so we were able to obtain reliable kinetic
parameter estimates. Box plots of Km,
Vmax and Clin,mic for liver and
small intestine are shown in figure 3.
Median Km values were 3.7, 3.8, 3.7 and 4.5 for
liver, duodenum, jejunum and ileum, respectively. ANOVA revealed no
differences in Km values among the four tissues
(P = .15). Moreover, no statistical difference was found if the
liver data were excluded from the analysis (P > .05 for all
pairwise comparisons). Median Vmax values were
850, 644, 426 and 68 pmol/min/mg for liver, duodenum, jejunum and
ileum, respectively. Not surprisingly, ANOVA revealed a statistically significant difference in Vmax among the four
tissues (P = .0001). With Dunn's test, only the ileum-liver
difference was significant. However, Wilcoxon signed-rank tests
revealed a significant difference between duodenum and ileum (P = .002) and jejunum and ileum (P = .005), but not between duodenum
and jejunum (P = .14). Median intrinsic clearances
(Clin,mic) for liver, duodenum, jejunum and ileum were 200, 157, 85 and 14 µl/min/mg. ANOVA with subsequent Dunn's test and
Wilcoxon signed-rank tests revealed similar contrasts as those
described for Vmax.
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Distribution of intestinal CYP3A, cytochrome
b5 and CYP reductase activities.
To
further define the CYP3A gradient along the entire small intestine and
determine the role of coenzymes in the regional variation of CYP3A
activity, the following were measured along the entire length of six
small intestines (HI-29, -30, -31, -32, -33 and -35): CYP3A catalytic
activity (1-OH MDZ formation rate), CYP3A protein content, NADPH- and
NADH-dependent cytochrome c reduction rates (as measures of
CYP reductase and cytochrome b5 reductase
activity, respectively) and cytochrome b5
protein content. For four of six intestines (HI-30, -32, -33 and -35),
CYP3A catalytic activity increased from duodenum to middle jejunum and
then decreased to distal ileum (fig. 4).
For HI-31, activity was highest in the first 1-foot section (duodenum)
and declined thereafter. For HI-29, activity was low for the first 5 to
6 feet of bowel, increased dramatically in midjejunum and declined
thereafter. Fold-differences between the section with the highest
activity vs. that with the lowest activity (distal ileum in
all cases) were 3-fold (HI-31 and HI-35) to 14-fold (HI-29, excluding
duodenum; HI-32) to 25-fold (HI-30 and HI-33). Intraintestinal
variability in CYP3A protein content was much less than that for CYP3A
activity and ranged from 1.5-fold (HI-31) to 4.6-fold (HI-30).
Correlations between CYP3A activity and protein content within an
intestine were significant for only four of the six intestines (HI-30,
-32, -33 and -35; rs = .83, .98, .71 and .90, respectively).
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1-OH MDZ to 4-OH MDZ ratios.
MDZ metabolite ratios (1-OH
MDZ/4-OH MDZ) were measured in microsomes prepared from six jejunums
and six livers. Three livers and three intestines with the highest
CYP3A5/CYP3A4 IOD ratios (HI-30, -31 and -35 and HL-125, -127 and -150)
were selected and compared with randomly chosen CYP3A5-negative organs
(HI-19, -20 and -28 and HL-107, -122 and -148). Results are summarized
in table 2. Ratios for CYP3A5-positive
jejunums were higher than CYP3A5-negative jejunums at all four
substrate concentrations examined. Interestingly, the jejunum with the
highest CYP3A5/CYP3A4 IOD ratio (0.64 for HI-30) had the highest
product ratio at all substrate concentrations. Product ratios for
CYP3A5-positive livers were also higher than CYP3A5-negative livers at
all four substrate concentrations examined (except for HL-125 at 0.25 µM MDZ). Mean product ratios for CYP3A5-negative livers were similar
to the corresponding ratios for CYP3A5-negative jejuna. In contrast, the mean product ratios for CYP3A5-positive livers were greater than
the corresponding ratios for CYP3A5-positive jejuna.
|
Total regional intestinal intrinsic clearances and scaling factors. Total intrinsic clearances for duodenum, jejunum and ileum (Clin,region) were estimated using microsomal intrinsic clearance (Clin,mic), microsomal CYP3A content and total regional CYP3A data. Total regional CYP3A was calculated using total wet weights of each region, mucosal recovery (as percent of tissue wet weight) and mucosal CYP3A content (based on corrected homogenate CYP3A content and homogenate mass/g mucosa). Because we had incomplete data collection, median values for microsomal intrinsic clearance (n = 15), microsomal CYP3A content (n = 20), regional wet weight (n = 7), mucosal recovery (n = 7) and mucosal CYP3A content (n = 10) were used for our calculations. Median regional wet weights were 79, 411 and 319 g for duodenum, jejunum and ileum, respectively. Mucosal masses represented 23%, 16% and 12% of total wet weights. Total median CYP3A contents were 445, 463 and 391 pmol/g mucosa, or 102, 74 and 47 pmol/g wet weight. Total regional CYP3A was thus 9.7, 38.4 and 22.4 nmol for duodenum, jejunum and ileum, respectively (fig. 6). Median Clin,mic values were 157, 85 and 14 µl/min/mg. Therefore, from equation 2, Clin,region values were calculated to be 50.1, 144.3 and 19.3 ml/min, respectively. The sum of these three values, total gut intrinsic clearance, was 213.7 ml/min. For comparison, we calculated total hepatic CYP3A to be 5490 nmol (69.7 pmol CYP3A/mg × 52.5 mg/g × 1500 g × 1 nmol/1000 pmol) and an intrinsic clearance of 15.8 l/min (0.2 ml/min/mg × 52.5 mg/g × 1500 g × 1 liter/1000 ml).
|
| |
Discussion |
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Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
Results from this study provide the first comprehensive
characterization of intraintestinal and interintestinal variability in
CYP3A expression and metabolic function. Although previous studies
involved either a limited sample size (De Waziers et al., 1990; McKinnon et al., 1995; Peters and Kremers, 1989;
Prueksaritanont et al., 1996; Thummel et al.,
1996) or collection of duodenal tissue only (Kivisto et al.,
1996; Lown et al., 1994), we examined 20 full-length
intestines. Nearly all were obtained from donors who had been
hospitalized for no more than 4 days before procurement (one donor,
HI-33, was hospitalized for 12 days). The organs were also procured
under carefully controlled conditions, with a limited period of cold
ischemia time and no warm ischemia time. Thus, although not identical
to biopsy tissue from healthy volunteers, we believe that potential
differences between donor and biopsy tissue with respect to mucosal
CYP3A stability (protein content and catalytic activity) were kept to a
minimum.
Our findings that CYP3A is the major cytochrome P450 expressed in all
three regions of the human small intestine fully agree with results
reported by Watkins et al. (1987) and De Waziers et
al. (1990). In contrast, CYP3A represented a smaller percentage of
total hepatic CYP compared with the mean percentage reported by Shimada
et al. (1994) (17% vs. 29%). For a fairer
comparison, we calculated a mean percentage of 20%, which is still
lower than the estimate of previous investigators. The discrepancy is
due to a slightly higher mean total CYP content and a lower mean CYP3A content observed in the present study compared with those from the
earlier study (0.38 vs. 0.34 nmol/mg and 83 vs.
96 pmol/mg, respectively). Nevertheless, small intestinal CYP3A
represents a larger percentage of total small intestinal CYP compared
with hepatic CYP3A as a percentage of total hepatic CYP.
We found large interindividual variability in CYP3A content for all
three regions of the small intestine, supporting the findings reported
by Lown et al. (1994), who measured CYP3A content in 20 duodenal pinch biopsies. Moreover, we corroborated the results reported
by De Waziers et al. (1990), who observed a progressive decline in microsomal CYP3A content from duodenum to jejunum to ileum.
The regional differences we observed, however, were not as great. The
previous investigators relied on small and uneven sample sizes
(n = 2, 6 and 5 for duodenum, jejunum and ileum, respectively); thus, larger interregional differences and a lower interindividual variability were observed. In contrast, the ranges of
CYP3A content we observed for different donors were considerable (3-90, 2-98 and 2-38 pmol/mg for duodenum, jejunum, and ileum, respectively) and are likely to be even larger because we were not able
to accurately quantify some very faint protein bands. The source of
this interindividual variability is not completely known. It could not
be explained by length of hospitalization, prior drug therapy, age or
sex of the donor population. Therefore, based on the similar degree of
variability in the present study, in which the intestinal mucosae had
been largely unexposed to potential dietary modulators for at least 48 hr before procurement, and that reported for duodenal biopsies from
healthy volunteers (Lown et al., 1994), we speculate that
these interindividual differences are derived largely from homeostatic
mechanisms (e.g., enterocyte differentiation, hormonal
control of gene expression and enterocyte turnover).
Rates of intestinal NADPH-dependent cytochrome c reduction
(range, 12-150 nmol/min/mg across all sections of the six intestines studied) agreed with those reported for 54 liver microsomal
preparations (Schmucker et al., 1990; range, 38-135
nmol/min/mg) and six ileal microsomal preparations (Pacifici et
al., 1989; range, 32-106 nmol/min/mg). Interestingly, HI-33 had
the lowest CYP reductase activity, <30 nmol/min/mg for all sections,
which may explain why this intestine had low CYP3A activity despite
moderate CYP3A content. Furthermore, the three most proximal and one
most distal section of HI-29 and the four ileal sections of HI-30 also
had low CYP reductase activity (<30 nmol/min/mg). Again, this may explain why we were not able to obtain kinetic parameter estimates from
some regions of these intestines.
With respect to intraintestinal comparisons, a significant correlation between CYP3A content and catalytic activity was observed for four of the six full-length organs examined, indicating that for the majority of individuals, enzyme function parallels protein content. Low intraintestinal variability in CYP3A content and activity (HI-31) or low CYP reductase activity (HI-29) may explain the poor correlations observed for the remaining two intestines. Furthermore, correlations between duodenal and jejunal Vmax (rs = .81) or Clin,mic (rs = .76) for the larger set of 15 donors were highly significant (P < 0.0001), suggesting that for most subjects, an analysis of duodenal pinch biopsies will provide representative metabolic information for the entire proximal intestine.
1-OH MDZ was the dominant metabolite in all intestine and liver
microsomal preparations and at all MDZ concentrations examined (0.25-8.0 µM). This is in agreement with previous reports of high 1-/4-OH MDZ ratios for hepatic microsomes when substrate
concentrations were <10 µM (Gorski et al., 1994; Kronbach
et al., 1989). Collectively, these in vitro
findings are consistent with in vivo observations (Heizmann
and Ziegler, 1981) that the 4-hydroxylation pathway contributes little
to the systemic metabolism of MDZ in vivo because plasma MDZ
concentrations are typically well below 1 µM.
The similarity in Km values for MDZ
1-hydroxylation (~4 µM) for the three intestinal regions and
liver, together with strong correlations between
Vmax and CYP3A content in both organs (except for ileum), suggest that hepatic and proximal gut CYP3A are
functionally equivalent. Although not statistically different, ileal
Km values tended to be higher than corresponding
duodenal and jejunal values. This, along with a poor correlation
between ileal Vmax and CYP3A content, implies
that ileal CYP3A behaves differently from more proximal CYP3A. Data
from our longitudinal studies further support this belief, where median
ileal CYP3A activity decreased to a greater extent than did CYP3A
content (fig. 5). Median, normalized CYP3A activity decreased 42% from
sections 11 to 13 and 47% from sections 13 to 15, whereas CYP3A
content decreased 10% and 19%, respectively. Overall, the data
indicate a much lower metabolic capacity for the distal compared with
the proximal small intestine.
Although we observed a 1-in-5 frequency of CYP3A5 expression in both
small intestine and liver, Lown et al. (1994) reported a
frequency of 70% for small intestine, and Jounaïdi et
al. (1996) reported a frequency of 74% for liver. This
discrepancy is likely due to different protein detection methods (the
other investigators used the more sensitive enhanced chemiluminescence
technique plus prolonged exposure). Nevertheless, in agreement with
these earlier studies, CYP3A5 was generally a minor component of total
CYP3A, which intimates that for most individuals, CYP3A5 plays a minor role in the intestinal and hepatic first-pass extraction of CYP3A substrates in vivo.
Before our analysis of matched liver and small intestinal tissue, we
expected the factors regulating the maintenance of CYP3A5 protein in a
given individual to be operative in both organs. This did not always
appear to be the case, however. The one discordant pair exhibited a
clear immunoreactive CYP3A5 band for liver but not for intestine.
Although the reason for this is unclear, it is possible that this
intestine received an insult either before or during procurement,
leading to enzyme degradation and a decrease in CYP3A5 below the limit
of detection. Interestingly, for the two intestines in which the CYP3A5
band was quantifiable (HI-30 and HI-31), the CYP3A5-to-CYP3A4 ratio
decreased from duodenum to jejunum and then increased in ileum to
values comparable to or greater than those observed for the duodenum.
This is consistent with previous reports of predominantly CYP3A5
expression in the stomach and colon (Gervot et al., 1996;
Kolars et al., 1994; Peters and Kremers, 1989).
There was no clear trend between the eight matched livers and
intestines with respect to MDZ 1-hydroxylation; that is, if the liver
had a high Clin,mic, the intestine did not necessarily have
a high Clin,mic. An extreme case is the pair HL-147 and
HI-26, where the liver exhibited one of the highest hepatic
Vmax and Clin,mic values and the
intestine had virtually no metabolic activity. Another case is the pair
HL-148 and HI-27, where the liver had moderately high
Vmax and Clin,mic values and the
intestine had low Vmax and Clin,mic
values. Some pairs did exhibit parallel CYP3A activities, such as
HL-146/HI-24 and HL-150/HI-30. Collectively, these findings support
in vivo observations reported by others (Lown et
al., 1994), who found that hepatic and intestinal CYP3A (measured
as the erythromycin breath test and 1-OH MDZ formation in duodenal
biopsies, respectively) are not coordinately regulated.
We estimated the duodenum to contain almost half the amount of CYP3A
compared with the ileum (9.7 vs. 22 nmol), which is striking given that the ileum is ~10 times longer than the duodenum (~10 feet vs. 1 foot; Snyder et al., 1975). The
discrepancy lies in the duodenal mucosa being extremely rich in villi,
the tips of which are lined with mature CYP3A-containing enterocytes.
The jejunum, whose villus density gradually decreases from proximal to
distal ends, is ~8 times longer than the duodenum and thus has the
greatest total amount of CYP3A. Total intrinsic clearances followed a
similar trend except that the duodenal value was higher than the ileal
value (50 vs. 19 ml/min). Again, this is reflective of a
metabolically active duodenum and a relatively deficient ileum.
Because the total hepatic intrinsic clearance was >70 times that for
the small intestine (15.8 and 0.21 l/min for liver and intestine,
respectively), it appears that the gut should contribute very little to
the metabolism of MDZ in vivo. However, recent studies
provide convincing evidence that both organs contribute equally, on
average, to the first-pass metabolism of this drug (Paine et
al., 1996; Thummel et al., 1996). Although unbound
intrinsic clearance is an important determinant of first-pass
extraction by both the liver and intestine, there is no a
priori reason to believe that the relationships between the
extraction ratio and the unbound intrinsic clearance, organ blood flow
and plasma protein binding should be the same for all organs of
elimination (Wilkinson, 1987). The effect of plasma protein binding and
hepatic blood flow on hepatic extraction is fairly well defined, but
their impact on gut extraction is unclear. Although exposure of
absorbed drug molecules to enterocytic CYP3A might be obligatory for
drugs absorbed transcellularly, drug access to hepatic CYP3A depends on
the translocation of unbound drug molecules across the sinusoidal
membrane into the parenchymal cell. In addition, although blood flow
should govern the residence time of drug molecules in the sinusoid and in the intestinal villus, limiting their exposure to CYP3A, the ratio
of blood flow to intrinsic clearance may be greater for liver than for
the intestinal mucosa.
If we assume a liver plasma flow of 0.78 l/min (MDZ does not partition
appreciably into erythrocytes), an unbound fraction of 0.02 (Thummel
et al., 1996) and a total hepatic unbound intrinsic clearance of 15.8 l/min and apply these to the well-stirred model for
hepatic clearance (Rowland et al., 1973), an in
vivo 1-OH MDZ formation clearance of 0.23 l/min was predicted. By
performing the same calculations for small intestine and assuming a
total wet weight of 809 g, a mucosal plasma flow of 0.16 l/min
(Hultén et al., 1977), the same unbound fraction and a
total unbound intrinsic clearance of 0.21 l/min, an in vivo
systemic clearance of 4.1 × 103 l/min was
predicted. This, together with the predicted hepatic 1-OH MDZ
formation clearance (0.23 l/min) being in excellent agreement with the
average and median systemic formation clearance we observed in healthy
volunteers (0.26 and 0.24 l/min, respectively; Thummel et
al., 1996), confirms our finding that the gut contributes little
to the systemic clearance of MDZ (Paine et al., 1996).
In vivo organ extraction ratios based on systemic delivery
of drug were predicted to be 0.29 and 0.03 for liver and small intestine, respectively. Both are within the range of values observed after intravenous administration (Paine et al., 1996;
Thummel et al., 1996). Pond and Tozer (1984) and Mistry and
Houston (1987) have suggested that the same relationship for intestinal
systemic extraction should apply to intestinal first-pass extraction.
However, the gut prediction is >10 times lower than the average
first-pass extraction ratio observed after intraduodenal administration
(0.43; Paine et al., 1996). If the unbound fraction is
excluded from the gut calculation, the extraction ratio increases to
0.57, which is closer to the first-pass gut extraction ratio observed
in vivo. This suggests that although plasma protein binding
reduces the efficiency of systemic intestinal MDZ extraction, it plays
a negligible role in determining the first-pass intestinal extraction
of the drug.
In summary, our extensive characterization of intestinal CYP3A metabolic capacity revealed that interorgan variability is much greater than intraorgan variability with respect to CYP3A expression and catalytic activity. This may account for the large interindividual differences observed in the oral bioavailabilities of some CYP3A substrates. Furthermore, our findings indicate that the upper small intestine (duodenum and proximal jejunum) serves as the major site for intestinal first-pass metabolism of midazolam and possibly immediate-release preparations (e.g., solutions, suspensions, uncoated tablets and capsules) of other CYP3A substrates that exhibit poor and unpredictable bioavailabilities. Alternatively, the low metabolic capacity of the ileum implies that slow-release preparations may largely be "spared" an intestinal first-pass effect. Finally, a comparison of predicted extraction ratios for the small intestine and liver suggests that protein binding, a factor that greatly influences the in vivo metabolism of several CYP3A substrates by the liver, does not apply to first-pass metabolic extraction by the intestine.
| |
Acknowledgments |
|---|
The authors wish to thank the Northwest Organ Procurement Agency for their assistance in the collection of donor tissues.
| |
Footnotes |
|---|
Accepted for publication August 27, 1997.
Received for publication April 28, 1997.
1 This work was supported in part by National Institutes of Health Grants GM48349, GM32165 and ES07033 and a fellowship from the American Foundation for Pharmaceutical Education.
Send reprint requests to: Kenneth E. Thummel, Ph.D., Department of Pharmaceutics, Box 357610, University of Washington, Seattle, WA 98195.
| |
Abbreviations |
|---|
CYP, cytochrome P450;
MDZ, midazolam;
1-OH
MDZ, 1-hydroxymidazolam;
4-OH MDZ, 4-hydroxymidazolam;
S9, supernatant
fraction at 9000 × g;
SDS, sodium dodecyl sulfate;
PAGE, polyacrylamide gel electrophoresis;
TEMED, N,N,N,N-tetra-methyl-ethylenediamine;
BCIP-NBT, 5-bromo-4-chloro-3-indoyl phosphate and nitroblue tetrazolium;
IOD, integrated optical density;
PMSF, phenylmethylsulfonyl fluoride;
EDTA, ethylenediamine tetraacetic acid;
ANOVA, analysis of variance.
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References |
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Abstract
Introduction
Methods
Results
Discussion
References
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M. F. Paine, S. S. Ludington, M.-L. Chen, P. W. Stewart, S.-M. Huang, and P. B. Watkins DO MEN AND WOMEN DIFFER IN PROXIMAL SMALL INTESTINAL CYP3A OR P-GLYCOPROTEIN EXPRESSION? Drug Metab. Dispos., March 1, 2005; 33(3): 426 - 433. [Abstract] [Full Text] [PDF]
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M. P. Duarte, B. B. Palma, A. A. Gilep, A. Laires, J. S. Oliveira, S. A. Usanov, J. Rueff, and M. Kranendonk The stimulatory role of human cytochrome b5 in the bioactivation activities of human CYP1A2, 2A6 and 2E1: a new cell expression system to study cytochrome P450 mediated biotransformation Mutagenesis, March 1, 2005; 20(2): 93 - 100. [Abstract] [Full Text] [PDF]
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M. F. Paine, A. B. Criss, and P. B. Watkins Two Major Grapefruit Juice Components Differ in Time to Onset of Intestinal CYP3A4 Inhibition J. Pharmacol. Exp. Ther., March 1, 2005; 312(3): 1151 - 1160. [Abstract] [Full Text] [PDF]
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 L. Quintieri, C. Geroni, M. Fantin, R. Battaglia, A. Rosato, W. Speed, P. Zanovello, and M. Floreani Formation and Antitumor Activity of PNU-159682, A Major Metabolite of Nemorubicin in Human Liver Microsomes Clin. Cancer Res., February 15, 2005; 11(4): 1608 - 1617. [Abstract] [Full Text] [PDF]
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A. Galetin, C. Brown, D. Hallifax, K. Ito, and J. B. Houston UTILITY OF RECOMBINANT ENZYME KINETICS IN PREDICTION OF HUMAN CLEARANCE: IMPACT OF VARIABILITY, CYP3A5, AND CYP2C19 ON CYP3A4 PROBE SUBSTRATES Drug Metab. Dispos., December 1, 2004; 32(12): 1411 - 1420. [Abstract] [Full Text] [PDF]
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W. Huang, Y. S. Lin, D. J. McConn II, J. C. Calamia, R. A. Totah, N. Isoherranen, M. Glodowski, and K. E. Thummel EVIDENCE OF SIGNIFICANT CONTRIBUTION FROM CYP3A5 TO HEPATIC DRUG METABOLISM Drug Metab. Dispos., December 1, 2004; 32(12): 1434 - 1445. [Abstract] [Full Text] [PDF]
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D. J. McConn II, Y. S. Lin, K. Allen, K. L. Kunze, and K. E. Thummel DIFFERENCES IN THE INHIBITION OF CYTOCHROMES P450 3A4 AND 3A5 BY METABOLITE-INHIBITOR COMPLEX-FORMING DRUGS Drug Metab. Dispos., October 1, 2004; 32(10): 1083 - 1091. [Abstract] [Full Text] [PDF]
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M. F. Paine, A. B. Criss, and P. B. Watkins TWO MAJOR GRAPEFRUIT JUICE COMPONENTS DIFFER IN INTESTINAL CYP3A4 INHIBITION KINETIC AND BINDING PROPERTIES Drug Metab. Dispos., October 1, 2004; 32(10): 1146 - 1153. [Abstract] [Full Text] [PDF]
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 E. L. Abel, S. M. Opp, C. L. M. J. Verlinde, T. K. Bammler, and D. L. Eaton Characterization of Atrazine Biotransformation by Human and Murine Glutathione S-Transferases Toxicol. Sci., August 1, 2004; 80(2): 230 - 238. [Abstract] [Full Text] [PDF]
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Y. Yasunami, H. Hara, T. Iwamura, T. Kataoka, and T. Adachi C-JUN N-TERMINAL KINASE MODULATES 1,25-DIHYDROXYVITAMIN D3-INDUCED CYTOCHROME P450 3A4 GENE EXPRESSION Drug Metab. Dispos., July 1, 2004; 32(7): 685 - 688. [Abstract] [Full Text] [PDF]
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J. S. Warrington, D. J. Greenblatt, and L. L. von Moltke The Effect of Age on P-Glycoprotein Expression and Function in the Fischer-344 Rat J. Pharmacol. Exp. Ther., May 1, 2004; 309(2): 730 - 736. [Abstract] [Full Text] [PDF]
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S. J. Mouly, M. F. Paine, and P. B. Watkins Contributions of CYP3A4, P-glycoprotein, and Serum Protein Binding to the Intestinal First-Pass Extraction of Saquinavir J. Pharmacol. Exp. Ther., March 1, 2004; 308(3): 941 - 948. [Abstract] [Full Text] [PDF]
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T. Morimoto, T. Kotegawa, K. Tsutsumi, Y. Ohtani, H. Imai, and S. Nakano Effect of St. John's Wort on the Pharmacokinetics of Theophylline in Healthy Volunteers J. Clin. Pharmacol., January 1, 2004; 44(1): 95 - 101. [Abstract] [Full Text] [PDF]
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K. S. Pang MODELING OF INTESTINAL DRUG ABSORPTION: ROLES OF TRANSPORTERS AND METABOLIC ENZYMES (FOR THE GILLETTE REVIEW SERIES) Drug Metab. Dispos., December 1, 2003; 31(12): 1507 - 1519. [Full Text] [PDF]
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L. S. Kaminsky and Q.-Y. Zhang THE SMALL INTESTINE AS A XENOBIOTIC-METABOLIZING ORGAN Drug Metab. Dispos., December 1, 2003; 31(12): 1520 - 1525. [Full Text] [PDF]
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J. C. Stevens, R. N. Hines, C. Gu, S. B. Koukouritaki, J. R. Manro, P. J. Tandler, and M. J. Zaya Developmental Expression of the Major Human Hepatic CYP3A Enzymes J. Pharmacol. Exp. Ther., November 1, 2003; 307(2): 573 - 582. [Abstract] [Full Text] [PDF]
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M. L. Veronese, L. P. Gillen, E. P. Dorval, W. W. Hauck, S. A. Waldman, and H. E. Greenberg Effect of Mibefradil on CYP3A4 In Vivo J. Clin. Pharmacol., October 1, 2003; 43(10): 1091 - 1100. [Abstract] [Full Text] [PDF]
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 W. P. D. Lemahieu, B. D. Maes, Y. Ghoos, P. Rutgeerts, K. Verbeke, and Y. Vanrenterghem Measurement of hepatic and intestinal CYP3A4 and PGP activity by combined po + iv [14C]erythromycin breath and urine test Am J Physiol Gastrointest Liver Physiol, August 8, 2003; 285(3): G470 - G482. [Abstract] [Full Text] [PDF]
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K. Ito, K. Ogihara, S.-i. Kanamitsu, and T. Itoh PREDICTION OF THE IN VIVO INTERACTION BETWEEN MIDAZOLAM AND MACROLIDES BASED ON IN VITRO STUDIES USING HUMAN LIVER MICROSOMES Drug Metab. Dispos., July 1, 2003; 31(7): 945 - 954. [Abstract] [Full Text] [PDF]
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S. Tamura, Y. Tokunaga, R. Ibuki, G. L. Amidon, H. Sezaki, and S. Yamashita The Site-Specific Transport and Metabolism of Tacrolimus in Rat Small Intestine J. Pharmacol. Exp. Ther., July 1, 2003; 306(1): 310 - 316. [Abstract] [Full Text] [PDF]
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A. Westlind-Johnsson, S. Malmebo, A. Johansson, C. Otter, T. B. Andersson, I. Johansson, R. J. Edwards, A. R. Boobis, and M. Ingelman-Sundberg COMPARATIVE ANALYSIS OF CYP3A EXPRESSION IN HUMAN LIVER SUGGESTS ONLY A MINOR ROLE FOR CYP3A5 IN DRUG METABOLISM Drug Metab. Dispos., June 1, 2003; 31(6): 755 - 761. [Abstract] [Full Text] [PDF]
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C. P. Granvil, A.-M. Yu, G. Elizondo, T. E. Akiyama, C. Cheung, L. Feigenbaum, K. W. Krausz, and F. J. Gonzalez Expression of the Human CYP3A4 Gene in the Small Intestine of Transgenic Mice: In Vitro Metabolism and Pharmacokinetics of Midazolam Drug Metab. Dispos., May 1, 2003; 31(5): 548 - 558. [Abstract] [Full Text] [PDF]
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D. Tam, R. G. Tirona, and K. S. Pang Segmental Intestinal Transporters and Metabolic Enzymes on Intestinal Drug Absorption Drug Metab. Dispos., April 1, 2003; 31(4): 373 - 383. [Abstract] [Full Text] [PDF]
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C. L. Cummins, L. Salphati, M. J. Reid, and L. Z. Benet In Vivo Modulation of Intestinal CYP3A Metabolism by P-Glycoprotein: Studies Using the Rat Single-Pass Intestinal Perfusion Model J. Pharmacol. Exp. Ther., April 1, 2003; 305(1): 306 - 314. [Abstract] [Full Text]
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T. S. Poet, H. Wu, A. A. Kousba, and C. Timchalk In Vitro Rat Hepatic and Intestinal Metabolism of the Organophosphate Pesticides Chlorpyrifos and Diazinon Toxicol. Sci., April 1, 2003; 72(2): 193 - 200. [Abstract] [Full Text] [PDF]
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P. S. Burton, J. T. Goodwin, T. J. Vidmar, and B. M. Amore Predicting Drug Absorption: How Nature Made It a Difficult Problem J. Pharmacol. Exp. Ther., December 1, 2002; 303(3): 889 - 895. [Abstract] [Full Text] [PDF]
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 C.M.F. Kruijtzer, J.H. Beijnen, and J.H.M. Schellens Improvement of Oral Drug Treatment by Temporary Inhibition of Drug Transporters and/or Cytochrome P450 in the Gastrointestinal Tract and Liver: An Overview Oncologist, December 1, 2002; 7(6): 516 - 530. [Abstract] [Full Text] [PDF]
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 R. H.N. van Schaik, I. P. van der Heiden, J. N. van den Anker, and J. Lindemans CYP3A5 Variant Allele Frequencies in Dutch Caucasians Clin. Chem., October 1, 2002; 48(10): 1668 - 1671. [Abstract] [Full Text] [PDF]
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 T. N. Johnson, A. Rostami-Hodjegan, J. M. Goddard, M. S. Tanner, and G. T. Tucker Contribution of midazolam and its 1-hydroxy metabolite to preoperative sedation in children: a pharmacokinetic-pharmacodynamic analysis Br. J. Anaesth., September 1, 2002; 89(3): 428 - 437. [Abstract] [Full Text] [PDF]
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Y. S. Lin, A. L. S. Dowling, S. D. Quigley, F. M. Farin, J. Zhang, J. Lamba, E. G. Schuetz, and K. E. Thummel Co-Regulation of CYP3A4 and CYP3A5 and Contribution to Hepatic and Intestinal Midazolam Metabolism Mol. Pharmacol., July 1, 2002; 62(1): 162 - 172. [Abstract] [Full Text] [PDF]
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L. Y. Li, G. L. Amidon, J. S. Kim, T. Heimbach, F. Kesisoglou, J. T. Topliss, and D. Fleisher Intestinal Metabolism Promotes Regional Differences in Apical Uptake of Indinavir: Coupled Effect of P-Glycoprotein and Cytochrome P450 3A on Indinavir Membrane Permeability in Rat J. Pharmacol. Exp. Ther., May 1, 2002; 301(2): 586 - 593. [Abstract] [Full Text] [PDF]
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M. F. Paine, L. Y. Leung, H. K. Lim, K. Liao, A. Oganesian, M.-Y. Zhang, K. E. Thummel, and P. B. Watkins Identification of a Novel Route of Extraction of Sirolimus in Human Small Intestine: Roles of Metabolism and Secretion J. Pharmacol. Exp. Ther., April 1, 2002; 301(1): 174 - 186. [Abstract] [Full Text] [PDF]
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K. E. Thummel, C. Brimer, K. Yasuda, J. Thottassery, T. Senn, Y. Lin, H. Ishizuka, E. Kharasch, J. Schuetz, and E. Schuetz Transcriptional Control of Intestinal Cytochrome P-4503A by 1alpha ,25-Dihydroxy Vitamin D3 Mol. Pharmacol., December 1, 2001; 60(6): 1399 - 1406. [Abstract] [Full Text] [PDF]
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Y. Oda and E. D. Kharasch Metabolism of Methadone and levo-alpha -Acetylmethadol (LAAM) by Human Intestinal Cytochrome P450 3A4 (CYP3A4): Potential Contribution of Intestinal Metabolism to Presystemic Clearance and Bioactivation J. Pharmacol. Exp. Ther., September 1, 2001; 298(3): 1021 - 1032. [Abstract] [Full Text] [PDF]
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K. Yoshisue, S. Nagayama, T. Shindo, and Y. Kawaguchi Effects of 5-Fluorouracil on the Drug-Metabolizing Enzymes of the Small Intestine and the Consequent Drug Interaction with Nifedipine in Rats J. Pharmacol. Exp. Ther., June 1, 2001; 297(3): 1166 - 1175. [Abstract] [Full Text]
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R. Yumoto, T. Murakami, M. Sanemasa, R. Nasu, J. Nagai, and M. Takano Pharmacokinetic Interaction of Cytochrome P450 3A-Related Compounds with Rhodamine 123, a P-Glycoprotein Substrate, in Rats Pretreated with Dexamethasone Drug Metab. Dispos., February 1, 2001; 29(2): 145 - 151. [Abstract] [Full Text]
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I. Kawahara, Y. Kato, H. Suzuki, M. Achira, K. Ito, C. L. Crespi, and Y. Sugiyama Selective Inhibition of Human Cytochrome P450 3A4 by N-[2(R)-Hydroxy-1(S)-indanyl]-5-[2(S)-(1,1-dimethylethylaminocarbonyl)-4-[(furo[2,3-b]pyridin-5-yl)methyl]piperazin-1-yl]-4(S)-hydroxy-2(R)-phenylmethylpentanamide and P-glycoprotein by Valspodar in Gene Transfectant Systems Drug Metab. Dispos., October 1, 2000; 28(10): 1238 - 1243. [Abstract] [Full Text] [PDF]
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C. K. Yeung, D. H. Lang, K. E. Thummel, and A. E. Rettie Immunoquantitation of FMO1 in Human Liver, Kidney, and Intestine Drug Metab. Dispos., September 1, 2000; 28(9): 1107 - 1111. [Abstract] [Full Text]
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 T. E. Lackner Advances in Managing Overactive Bladder Journal of Pharmacy Practice, August 1, 2000; 13(4): 277 - 289. [Abstract] [PDF]
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D. Cong, M. Doherty, and K. S. Pang A New Physiologically Based, Segregated-Flow Model to Explain Route-Dependent Intestinal Metabolism Drug Metab. Dispos., February 1, 2000; 28(2): 224 - 235. [Abstract] [Full Text]
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J. H. Hochman, M. Chiba, J. Nishime, M. Yamazaki, and J. H. Lin Influence of P-Glycoprotein on the Transport and Metabolism of Indinavir in Caco-2 Cells Expressing Cytochrome P-450 3A4 J. Pharmacol. Exp. Ther., January 1, 2000; 292(1): 310 - 318. [Abstract] [Full Text]
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W. Jacobsen, G. Kirchner, K. Hallensleben, L. Mancinelli, M. Deters, I. Hackbarth, K. Baner, L. Z. Benet, K.-F. Sewing, and U. Christians Small Intestinal Metabolism of the 3-Hydroxy-3-methylglutaryl-Coenzyme A Reductase Inhibitor Lovastatin and Comparison with Pravastatin J. Pharmacol. Exp. Ther., October 1, 1999; 291(1): 131 - 139. [Abstract] [Full Text]
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S. Ekins, G. Bravi, J. H. Wikel, and S. A. Wrighton Three-Dimensional-Quantitative Structure Activity Relationship Analysis of Cytochrome P-450 3A4 Substrates J. Pharmacol. Exp. Ther., October 1, 1999; 291(1): 424 - 433. [Abstract] [Full Text]
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Q.-Y. Zhang, D. Dunbar, A. Ostrowska, S. Zeisloft, J. Yang, and L. S. Kaminsky Characterization of Human Small Intestinal Cytochromes P-450 Drug Metab. Dispos., July 1, 1999; 27(7): 804 - 809. [Abstract] [Full Text]
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 J. H. Lin, M. Chiba, and T. A. Baillie Is the Role of the Small Intestine in First-Pass Metabolism Overemphasized? Pharmacol. Rev., June 1, 1999; 51(2): 135 - 158. [Abstract] [Full Text] [PDF]
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M. A. Gibbs, K. L. Kunze, W. N. Howald, and K. E. Thummel Effect of Inhibitor Depletion on Inhibitory Potency: Tight Binding Inhibition of CYP3A by Clotrimazole Drug Metab. Dispos., May 1, 1999; 27(5): 596 - 599. [Abstract] [Full Text]
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J. M. Fisher, S. A. Wrighton, P. B. Watkins, P. Schmiedlin-Ren, J. C. Calamia, D. D. Shen, K. L. Kunze, and K. E. Thummel First-Pass Midazolam Metabolism Catalyzed by 1alpha ,25-Dihydroxy Vitamin D3-Modified Caco-2 Cell Monolayers J. Pharmacol. Exp. Ther., May 1, 1999; 289(2): 1134 - 1142. [Abstract] [Full Text]
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J. M. Fisher, S. A. Wrighton, J. C. Calamia, D. D. Shen, K. L. Kunze, and K. E. Thummel Midazolam Metabolism by Modified Caco-2 Monolayers: Effects of Extracellular Protein Binding J. Pharmacol. Exp. Ther., May 1, 1999; 289(2): 1143 - 1150. [Abstract] [Full Text]
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M. F. Paine, P. Schmiedlin-Ren, and P. B. Watkins Cytochrome P-450 1A1 Expression in Human Small Bowel: Interindividual Variation and Inhibition by Ketoconazole Drug Metab. Dispos., March 1, 1999; 27(3): 360 - 364. [Abstract] [Full Text]
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M. A. Gibbs, K. E. Thummel, D. D. Shen, and K. L. Kunze Inhibition of Cytochrome P-450 3A (CYP3A) in Human Intestinal and Liver Microsomes: Comparison of Ki Values and Impact of CYP3A5 Expression Drug Metab. Dispos., February 1, 1999; 27(2): 180 - 187. [Abstract] [Full Text]
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, Outliers (values between 1.5 and 3 box-lengths from the upper or
lower edge). 
, Extremes (values >3 box-lengths from the upper or
lower edge). * Median significantly different from liver median (P < .05, Kruskal-Wallis). ** Median significantly different
from duodenal and jejunal medians (P < .01, Wilcoxon signed-rank
test). See text for explanation of statistical tests.
