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Vol. 282, Issue 2, 617-632, 1997
Division of Pharmaceutics and Biopharmaceutics,
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Abstract |
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 Top
Abstract
Introduction
Methods
Results
Discussion
References
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Previous estimates of maternal and fetal placental and
nonplacental clearances in pregnant sheep using a two-compartment open model have revealed higher values of fetal placental clearance (CLfm) compared to the maternal placental clearance
(CLmf) for most drugs. This includes the antihistamine
diphenhydramine (DPHM), which also has the highest weight-corrected
fetal nonplacental clearance (CLfo) among the drugs
studied. This study was designed to determine the reasons for this
CLfm 
CLmf difference and to identify the
sites of high CLfo for DPHM. DPHM and a stable
isotope-labeled analog, [2H10]DPHM, were
simultaneously infused to steady state to the mother and fetus,
respectively, in five pregnant sheep. CLmf,
CLfm, CLmo and CLfo averaged
50.3 ± 13.2, 214.4 ± 30.8, 36.6 ± 1.9 and 109.8 ± 22.3 ml/min
1/kg1,
respectively. By measuring diphenylmethoxyacetic acid and
[2H10]diphenylmethoxyacetic acid levels in
samples obtained from our previous study of fetal hepatic first-pass
DPHM uptake, the hepatic first-pass extraction ratio of the drug from
umbilical venous blood was estimated to be 0.44 ± 0.05. This can
account for virtually all of CLfo. Fetal hepatic first-pass
uptake of maternally derived DPHM in the paired infusion study reduces
the fetal/maternal plasma DPHM concentration ratio and results in significant underestimation of CLmf. When the
CLmf estimate is corrected for this factor and for
maternal-fetal DPHM plasma protein binding differences, its value
approaches CLfm. Fetal hepatic first-pass uptake may also
be a factor in the underestimation of CLmf for most of the
other drugs. Conversely, a lower value of CLmf compared
with CLfm provides evidence for significant fetal hepatic
uptake of these compounds.
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Introduction |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The
extent of fetal exposure to maternally administered drugs is determined
by a number of factors, including physicochemical characteristics of
the drug in question, permeability characteristics of the placenta and
the length of time the drug is present in the maternal circulation
(Reynolds and Knott, 1989
; Rurak et al., 1991). During
long-term administration with steady-state drug concentrations in the
mother, two additional factors become important in determining fetal
exposure: maternal and fetal plasma protein binding and fetal
nonplacental clearance of the drug. Szeto et al. (1982a)
have shown that under steady-state conditions, the fetal-to-maternal
drug concentration ratio during maternal drug administration is
determined by the maternal placental clearance divided by the sum of
fetal placental and nonplacental clearances (i.e.,
Cfss/Cmss = CLmf/[CLfm + CLfo]). Thus, when the fetus is able to eliminate the
drug via nonplacental routes, fetal drug exposure is
reduced.
Maternal and fetal placental and nonplacental clearances have been
determined for a number of drugs in pregnant sheep. The most commonly
used method is the two-compartment open model proposed by Szeto
et al. (1982a). This technique involves paired maternal and
fetal intravenous infusions of the drug to steady state and collection
of paired maternal and fetal plasma samples. From the infusion rates of
the drug and the maternal and fetal steady-state drug concentrations,
maternal and fetal placental (i.e., bidirectional) and
nonplacental clearance values can be estimated. To date, this method
has been used with morphine and methadone (Szeto et al., 1982b), acetaminophen (Wang et al., 1986), metoclopramide
(Riggs et al., 1990) and DPHM (Yoo et al., 1993).
With the exception of acetaminophen, all of the compounds studied thus
far have exhibited a higher value for CLfm compared to
CLmf. This has also been found with labetalol using a
different method to estimate maternal and fetal transplacental
clearances (Yeleswaram et al., 1993). Given that the
placental transfer of all these drugs appears to occur by passive
diffusion and that CLmf should equal CLfm (see
Discussion for further comment on this point), these findings are
surprising. Yoo et al. (1993) reported that the magnitude of
the CLfm CLmf difference is linearly related
to the fetal placental clearance. Of drugs studied to date, the
greatest difference between fetal and maternal placental clearance
occurs with the histamine antagonist DPHM, with the fetal clearance
value being 3.7 times that determined in the ewe (Yoo et
al., 1993). However, no explanation for this phenomenon appears to
have been provided in the literature. The weight-normalized DPHM
nonplacental clearance in the fetal lamb is also higher than the
corresponding maternal value, but the routes of fetal nonplacental
elimination have not been totally elucidated. This is also the case for
other drugs that have been studied in pregnant sheep.
We consider that there could be at least two possible explanations for
the higher value of fetal placental clearance. One relates to a
methodological issue. Ideally, the two-compartment model experimental
protocol should use simultaneous maternal and fetal drug infusions.
However, this requires a stable isotope-labeled analog of the drug and
an analysis method to quantify both forms of the drug when present
together in biological fluids. This was not possible in previous
studies, and time-separated maternal and fetal drug administration was
carried out. Although the order of drug administration was randomized,
it seems possible that with the rapid growth and maturation of the
fetus in late gestation, the time separation of the maternal and fetal
infusions could have artifactually affected the clearance estimates.
The other possibility involves fetal hepatic first-pass uptake of a
portion of the drug transferred to the fetus via placenta.
Drug administered to the mother reaches the fetus via the
umbilical vein (UV), and ~50% of UV flow enters the fetal liver
before reaching the fetal systemic circulation (Holzman, 1984). If
fetal hepatic drug uptake was significant, the fetal systemic
availability and plasma concentration of maternally administered drug
reaching the fetal systemic circulation would be reduced, and this
would result in an underestimation of maternal placental clearance.
Recently, however, we reported that there is no detectable hepatic
first-pass uptake of DPHM from the UV blood in the fetal lamb in a
study involving simultaneous UV and tarsal venous (TV) administration
of unlabeled and deuterium-labeled DPHM and measurement of the two
forms of drug in fetal systemic circulation (Tonn et al.,
1996).
The overall objective of the current study was to determine the reason
or reasons for the difference in maternal and fetal placental
clearances and to elucidate the components of high fetal nonplacental
clearance for DPHM. Because this drug exhibits the greatest
CLfm CLmf difference of all drugs studied in
pregnant sheep, an explanation for this difference could also be
relevant to other compounds. To achieve this objective, we reassessed
maternal and fetal clearances of DPHM using simultaneous maternal and
fetal infusions of unlabeled and stable isotope-labeled drug. We also reexamined fetal hepatic first-pass uptake of DPHM from the UV blood by
measuring the fetal plasma concentrations of the labeled and unlabeled
forms of a DPHM metabolite, DPMA, which has a very low placental
permeability in sheep compared to the parent drug. Using these data,
the contribution of fetal hepatic clearance to overall CLfo
was assessed; in addition, the maternal and fetal renal clearances of
DPHM and DPMA were measured. Finally, we assessed the impact of fetal
hepatic first-pass uptake of maternally derived DPHM on the estimates
of maternal and fetal clearance parameters calculated using the
two-compartment open model.
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Methods |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Animals and Surgical Preparation
This study was approved by the University of British Columbia Animal Care Committee, and all procedures performed on the sheep conformed to the guidelines of the Canadian Council on Animal Care. Five pregnant Dorset Suffolk cross-bred ewes, with a maternal body weight of 70.5 ± 3.4 kg (mean ± S.E.M.), were surgically prepared at 119 to 127 days gestation (122 ± 1 day, term ~145 days). Surgery was performed aseptically under halothane (1-2%) and nitrous oxide (60%) anesthesia (balance O2), after induction of anesthesia with intravenous sodium pentothal (1 g) and intubation of the ewe. Silicone rubber catheters (Dow Corning, Midland, MI) were implanted in FA and CA, common UV and lateral tarsal veins, trachea, urinary bladder (via a suprapubic incision) and the amniotic cavity. Electrodes (Cooper Corporation, Chatsworth, CA) were implanted biparietally on the dura to record the fetal electrocorticogram. In four animals, a transit-time 4SB blood flow transducer (Transonic Systems, Ithaca, NY) was placed around the common umbilical artery to measure umbilical blood flow. Catheters were also implanted in a maternal femoral artery (MA) and maternal femoral vein (MV). The catheters, electrodes and flow cables were tunneled subcutaneously to a small incision on the flank of the ewe where they exited. They were stored in a denim pouch when not in use. Each vascular catheter was flushed daily with ~2 ml of sterile 0.9% sodium chloride containing 12 units of heparin/ml to maintain catheter patency. Intramuscular injections of 500 mg of ampicillin and 80 mg of gentamicin were administered to the ewe on the day of surgery and for 3 days after surgery. Ampicillin (500 mg) and gentamicin (40 mg) were administered via the amniotic cavity immediately after surgery and then daily thereafter. After surgery, animals were kept in holding pens with other sheep and were given free access to food and water. The sheep were allowed to recover for 4 to 8 days before experimentation. On the morning of the experiment, a Foley bladder catheter was inserted via the urethra of the ewe and attached to a sterile polyvinyl bag for cumulative urine collection.
Experimental Protocol
Experiments were conducted at 125 to 133 days (128.8 ± 1.4 days) (term 145 days gestation). Before each experiment, DPHM · HCl (Sigma Chemical, St. Louis, MO) and
[2H10]DPHM · HCl (synthesized and
purified in our laboratory; Tonn et al., 1993) were weighed
to obtain the correct dose for administration. The weighed doses were
dissolved in sterile 0.9% sodium chloride for injection and then
filtered through a 0.22-µm nylon syringe filter (MSI, Westboro, MA)
into a capped empty sterile injection vial.
Two types of experiments (studies 1 and 2) were carried out on this group of animals, as described below.
Study 1: Fetal isotope effect studies.
These studies were
conducted on two animals to check for the presence of any isotope
effects in the disposition of [2H10]DPHM and
the metabolite [2H10]DPMA compared with DPHM
and DPMA. Equimolar doses of DPHM and
[2H10]DPHM were simultaneously administered
via the TV catheter as a 2.0-mg loading dose followed
immediately by a 90-min infusion (60 µg/min). Serial samples were
collected at 5, 5, 15, 30, 45, 60, 75 and 90 min from the FA and CA
(1.5 ml each) and MA (3.0 ml) catheters. Amniotic fluid and fetal urine
samples (3.0 ml) were also collected at 5, 30, 60 and 90 min.
Study 2: Paired maternal-fetal infusions.
Simultaneous
infusions of DPHM and [2H10]DPHM to the ewe
and fetus, respectively, were carried out on all five sheep. In the two
animals (animals E2241 and E2181) used for the isotope effect study,
the paired maternal-fetal infusions were carried out 72 hr later. DPHM
was administered as a 20-mg intravenous loading dose over 1.0 min,
followed immediately by an infusion of 670 µg/min via the
MV. Simultaneously, a 5.0-mg intravenous loading dose of
[2H10]DPHM was given via the TV
over 1.0 min, followed by an infusion of the compound at 170 µg/min.
Simultaneous blood samples were collected from the FA (1.5 ml) and MA
(3.0 ml) catheters at 5, 30, 60, 90, 120, 150, 180, 210, 240, 270, 300, 330 and 360 min during the infusion and at 30, 60, 120, 180, 240 and 360 min and 8, 12, 18, 24, 30 and 40 hr after the infusion. FA
samples (0.6 ml) were also collected at the same time intervals for
blood gas analysis and measurement of glucose and lactate
concentrations. CA and UV blood samples (1.5 ml) were collected at 5,
30, 60, 90, 120, 150, 180, 210, 240, 270, 300, 330 and 360 min during the infusion period. All fetal blood removed for sampling was replaced
at intervals during the experiment by an equal volume of maternal blood
obtained before the start of the experiment. Amniotic and tracheal
fluid (3.0 ml) and maternal urine (10 ml) samples were obtained at 5,
60, 120, 180, 240, 300 and 360 min during the infusion and at 60, 120, 180, 240 and 360 min and 8, 12, 18, 24, 30 and 40 hr postinfusion.
20°C until the time of analysis (
3
months from sample collection).
Study 3: Simultaneous fetal UV and tarsal venous
administration.
In addition to the studies described above, data
that we recently obtained using samples collected from eight animals
used in our previous study of fetal DPHM hepatic first-pass uptake (Tonn et al., 1996) are reported here. As noted in the
introduction, ~50% (range, 30-80%) of the UV flow traverses the
fetal liver before reaching the fetal systemic circulation (Edelstone
et al., 1978). Moreover, UV provides a major vascular input
into the fetal liver, supplying ~93% and ~60% of the total blood
flow to the left and the right and caudate lobes, respectively
(Edelstone et al., 1978; Holzman, 1984). Thus, the drug
present in UV could undergo a "partial" first-pass hepatic uptake
before entering the fetal circulation if the fetal liver was
sufficiently active in metabolizing the drug (fig.
1). The surgical preparation and experimental protocol used in these animals have been previously fully
described (Tonn et al., 1996). The surgery was similar to that described above, with the exception that fetal and maternal bladder catheters were not used. To assess the fetal first-pass hepatic
uptake for DPHM, we used simultaneous but separate bolus injections of
[2H10]DPHM and DPHM (5.0 mg each)
via the common UV and TV (which drains directly into the
inferior vena cava) or 90-min intravenous infusions of the compounds
(60 µg/min each, preceded by a 2.0 mg intravenous bolus of each)
via the same routes. This was coupled with collection of
fetal arterial plasma for the measurement of [2H10]DPHM and DPHM concentrations. In the
present study, fetal plasma samples remaining from four of these fetal
bolus and four of the infusion studies were used for the measurement of
[2H10]DPMA and DPMA concentrations.
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Physiological Recording and Monitoring Procedures
From 
24 hr before to 24 hr after the infusion period, fetal
amniotic, tracheal and FA pressures, heart rate, electrocortical activity and urine production rate were continuously monitored. However, these data will be reported separately. In the animals with an
implanted umbilical flow transducer, UV blood flow was measured with a
Transonic model T201 transit-time flowmeter (Transonic Systems, Inc.,
Ithaca, NY). Fetal urine flow rate was estimated using a
computer-controlled roller pump assembly developed in our laboratory.
The fetal bladder catheter was allowed to drain by gravity into a
sterile reservoir (10-ml syringe barrel) to which a disposable DTX
transducer was connected. When the pressure in the reservoir increased
above a preset level (usually 3 mm Hg) due to urine collection, the
computer activated a roller pump (DIAS Ex154, DIAS Inc., Kalamazoo,
MI), which pumped a calibrated volume of urine from the reservoir back
to the amniotic cavity (via the amniotic catheter) during
control periods. During the experimental period, the urine was
collected into a sterile sample collection syringe, and at hourly
intervals a 5-ml aliquot was taken, with the remainder of the urine
returned to the amniotic cavity. The cumulative volume pumped/min,
which equals fetal urine production/min, was stored on disk.
Blood pH, PO2 and PCO2 were measured using an IL 1306 pH/blood gas analyzer (Allied Instrumentation Laboratory, Milan, Italy). Blood O2 saturation and hemoglobin concentration were determined using a Hemoximeter (Radiometer, Copenhagen, Denmark). Blood glucose and lactate concentrations were determined with a 2300 STAT plus glucose/lactate analyzer (Y.S.I. Inc., Yellow Springs, OH).
Plasma Protein Binding of DPMA in Fetal and Maternal Plasma
The plasma protein binding of DPMA was measured in
vitro in fetal and maternal plasma using equilibrium dialysis as
described by Tonn et al. (1992). Maternal and fetal plasma
for these measurements was obtained from two additional sheep in our
laboratory set up for other experiments, and the drug-free plasma was
obtained on nonexperimental days.
Drug and Metabolite Analysis
The concentrations of DPHM and
[2H10]DPHM in all biological fluids collected
were measured using a previously developed GC-MS assay capable of
simultaneously measuring DPHM and [2H10]DPHM
(LOQ = 2 ng/ml each; Tonn et al., 1993). The
concentrations of DPMA and its stable isotope labeled analog,
[2H10]DPMA, were measured simultaneously
using another GC-MS method, which was also developed in our laboratory
(LOQ = 2.5 ng/ml each; Tonn et al., 1995).
Pharmacokinetic Analysis
Study 2: Paired maternal-fetal infusions.
The fetal and
maternal plasma concentration-vs.-time data from this study
were fit separately to a two-compartment open model with elimination
occurring from the central compartment (Gibaldi and Perrier, 1982). The
data were fit using ADAPT II pharmacokinetic modeling program and a
maximum likelihood fitting algorithm [variance model for Cp: Var = 
*(Cp) + 
, where and are estimated variance parameters]
(D'Argenio and Schumitzky, 1992). Plasma concentration at time 0 (Cp0) was extrapolated from the fitted equation.
). Clearances were calculated from the
equations 1 to 6 as previously described (Szeto et al.,
1982a).
![CL<SUB>mm</SUB><IT>=</IT><FR><NU><IT>k</IT><SUB><IT>o</IT></SUB></NU><DE>[C<SUB>mss</SUB><IT>−</IT>C<SUB>fss</SUB><IT>*</IT>(C<SUB>mss</SUB><IT>′/</IT>C<SUB>fss</SUB><IT>′</IT>)]</DE></FR>](/content/vol282/issue2/fulltext/617/img001.gif)
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(1) |
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(2) |
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(3) |
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(4) |
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(5) |
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(6) |
denote the drug infusion rates to the mother
(DPHM) and fetus ([2H10]DPHM), respectively.
Fetal DPHM placental clearance were also calculated using
the Fick method in two animals in which umbilical blood flow and the
concentrations of DPHM and [2H10]DPHM were
measured in paired samples of FA and fetal UV plasma. The purpose was
to assess whether placental metabolism could contribute to the high
fetal nonplacental clearance of the drug (Yoo et al., 1993)
because with the two-compartment model, placental drug metabolism on
the fetal side of placenta would appear as fetal nonplacental clearance
(Szeto et al., 1982a). The equation for Fick estimation is
given below:
![CL<SUB>fm</SUB><IT>=</IT>Q<SUB>um</SUB><IT>*</IT><FENCE><FR><NU>[(<SUP><IT>2</IT></SUP>H<SUB><IT>10</IT></SUB>)DPHM]<SUB>FA</SUB><IT>−</IT>[(<SUP><IT>2</IT></SUP>H<SUB><IT>10</IT></SUB>)DPHM]<SUB>UV</SUB></NU><DE>[(<SUP><IT>2</IT></SUP>H<SUB><IT>10</IT></SUB>)DPHM]<SUB>FA</SUB></DE></FR></FENCE>](/content/vol282/issue2/fulltext/617/img007.gif)
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(7) |
![ER<IT>=</IT><FR><NU>(AUC<SUB>DPMA</SUB><IT>/</IT>AUC<SUB>DPHM</SUB>)<IT>−</IT>(AUC<SUB>[<SUP>2</SUP>H<SUB>10</SUB>]DPMA</SUB><IT>/</IT>AUC<SUB>[<SUP>2</SUP>H<SUB>10</SUB>]DPHM</SUB>)</NU><DE>(AUC<SUB>DPMA</SUB><IT>/</IT>AUC<SUB>DPHM</SUB>)</DE></FR>](/content/vol282/issue2/fulltext/617/img008.gif)
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(8) |
):
![CL<SUB>ren(DPHM or [<SUP>2</SUP>H<SUB>10</SUB>]DPHM)</SUB><IT>=</IT><FR><NU>Xu<SUP><IT>∞</IT></SUP><SUB>(DPHM or [<SUP>2</SUP>H<SUB>10</SUB>]DPHM)</SUB></NU><DE>AUC<SUB><IT>0–∞ </IT>(DPHM or [<SUP>2</SUP>H<SUB>10</SUB>]DPHM)</SUB></DE></FR>](/content/vol282/issue2/fulltext/617/img009.gif)
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(9) |
![CL<SUB>ren(DPMA or [<SUP>2</SUP>H<SUB>10</SUB>]DPMA)</SUB><IT>=</IT><FR><NU>Xu<SUP><IT>∞</IT></SUP><SUB>(DPMA or [<SUP>2</SUP>H<SUB>10</SUB>]DPMA)</SUB></NU><DE>AUC<SUB><IT>0–∞ </IT>(DPMA or [<SUP>2</SUP>H<SUB>10</SUB>]DPMA)</SUB></DE></FR>](/content/vol282/issue2/fulltext/617/img010.gif)
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(10) |
is the total cumulative amount of DPHM
or DPMA excreted in the urine, and AUCs refer to respective area under
the plasma concentration-vs.-time curve of drug or
metabolite in the ewe or the fetus.
The contribution of maternal DPHM and fetal
[2H10]DPHM renal elimination to respective
DPHM nonplacental clearance was calculated as the ratio of their renal
clearance values to nonplacental clearance values (CLmo and
CLfo, respectively). The percentage of administered maternal DPHM and fetal [2H10]DPHM dose
excreted as DPMA and [2H10]DPMA in maternal
and fetal urine, respectively, was calculated from the ratio of
cumulative amount of unlabeled or labeled DPMA (corrected for mass
difference between parent drug and metabolite) excreted in the urine at
time infinity to the administered DPHM or
[2H10]DPHM dose.
Study 3: Simultaneous fetal UV and TV administration: For these fetal hepatic first-pass experiments, fetal systemic availability of DPHM (or [2H10]DPHM) after UV administration was calculated from the parent drug data as previously described (Tonn et al. , 1996):
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(11) |
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(12) |
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(13) |
or AUC0-tlast) for parent
drug or metabolite in all experiments were calculated using the linear
trapezoidal method (Gibaldi and Perrier, 1982).
Statistical analysis.
All values are reported as the
mean ± S.E.M. The achievement of steady state was determined
using three groups of mean concentration values (i.e., 150 and 180, 240 and 270, and 330 and 360 min) with a repeated-measures
analysis of variance (Zar, 1984). A paired t test was used
to test for differences between fetal and maternal pharmacokinetic
parameters. The significance level was P < .05 in all cases.
Fetal weight in utero at the time of experimentation was
estimated from the weight at birth and the time interval between the
experiment and birth (Koong et al., 1975).
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Results |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Study 1: Fetal Isotope Effect Studies
In two experiments, DPHM and [2H10]DPHM were simultaneously infused via the TV for 90 min to determine possible differences in the disposition of two forms of the drug. The overall mean steady-state plasma concentrations of DPHM and [2H10]DPHM in the two animals were 183.6 ± 30.9 and 182.4 ± 30.3 ng/ml, respectively. For DPMA and [2H10]DPMA, steady-state concentrations were not achieved during the infusion, but there were no apparent differences between the AUCs for DPMA (1598.2 ng.min/ml) and [2H10]DPMA (1429.5 ng.min/ml). In addition, no differences were observed in the concentrations of DPHM and [2H10]DPHM in maternal plasma (10.4 ± 0.5 vs. 11.0 ± 0.5 ng/ml), AUCs in amniotic fluid (1054.8 vs. 1101.0 ng.min/ml) and fetal urinary concentrations at the end (90 min) of the infusion (2944.0 vs. 2874.3 ng/ml). Overall, the data do not indicate any significant isotope effect in the disposition of labeled forms of DPHM and DPMA.
Study 2: Paired Maternal/Fetal Infusions
The five experiments involving the simultaneous 6-hr infusions of DPHM and [2H10]DPHM to ewe and fetus, respectively, were carried out at 125 to 133 days gestation (128.8 ± 1.4 days). Estimated fetal weight was 2.46 ± 0.09 kg. During the control period, the fetal femoral arterial values for pH, PO2, PCO2, O2 saturation, hemoglobin, glucose and lactate concentrations were 7.36 ± 0.02, 22.6 ± 1.65 mm Hg, 47.3 ± 0.5 mm Hg, 55.3 ± 23.8%, 10.0 ± 0.3 g/dl, 0.98 ± 0.09 mM and 0.70 ± 0.11 mM, respectively. There were no consistent changes in any of these variables during or after the infusion period. Likewise umbilical blood flow (281 ± 39 ml/min/kg, n = 3) was not consistently altered during the experiment.
Maternal and fetal plasma DPHM and
[2H10]DPHM concentrations and placental and
nonplacental clearance values.
The average plasma concentrations
of DPHM and [2H10]DPHM in MA and FA plasma
are illustrated in figure 2. They reached
a plateau at ~120 min, and there were no statistical differences
between the plasma concentrations at 150 and 180, 240 and 270, and 330 and 360 min, suggesting the achievement of steady state by 150 min.
Thus, mean steady-state concentration values used for subsequent calculations were taken from 150 to 360 min. The mean steady-state concentrations of DPHM were 260.8 ± 18.9 and 45.6 ± 17.4 ng/ml in MA and FA plasma, respectively, whereas the mean
concentrations of [2H10]DPHM in the same
vessels were 44.6 ± 5.8 and 244.0 ± 42.4 ng/ml,
respectively. The total MA and FA steady-state concentrations of DPHM
(i.e., labeled and unlabeled DPHM) were 305.4 ± 24.4 and 289.6 ± 57.6 ng/ml. In the four fetuses in which there was a
functional CA catheter, the mean concentrations of
[2H10]DPHM (infused via the tarsal
vein) were 203.7 ± 29.9 and 186.1 ± 27.0 ng/ml in FA and CA
plasma, respectively. The mean FA-CA concentration difference of
17.5 ± 6.1 ng/ml was significantly different from 0. In contrast,
the concentrations of DPHM (infused to the ewe) in FA and CA plasma
averaged 27.2 ± 4.4 and 26.6 ± 4.3 ng/ml in these four
animals and were not significantly different. As in previous studies
(Rurak et al., 1991), there was accumulation of DPHM (both
labeled and unlabeled) in fetal lung and amniotic fluids. The average
drug concentration ratio between lung fluid and FA plasma was 4.0 ± 1.7 for DPHM and 4.5 ± 1.6 for
[2H10]DPHM, whereas the corresponding ratios
in amniotic fluid (i.e., amniotic fluid/FA) were 0.6 ± 0.2 and 0.8 ± 0.2 for labeled and unlabeled drug, respectively.
After the infusion, concentrations of DPHM and
[2H10]DPHM in all fluids declined rapidly
with a terminal elimination half-life in plasma of 70.5 ± 6.9 and
51.8 ± 7.2 min in the ewe and fetus, respectively.
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Fetal and maternal DPMA and [2H10]DPMA
plasma concentrations.
A mean plasma
concentration-vs.-time plot of DPMA and
[2H10]DPMA in MA and FA plasma is shown in
figure 3. Although concentrations of DPHM
and [2H10]DPHM reached steady state at ~120
min from the start of the infusion (fig. 2), the plasma levels of DPMA
and [2H10]DPMA did not reach steady state
during the entire duration of infusion and continued to increase for 30 to 120 min after infusion. At all time points during the infusion
period, the concentration of [2H10]DPMA was
higher in the fetus than in the mother, whereas for the unlabeled
metabolite the situation was reversed. The peak concentrations of DPMA
in maternal and fetal plasma averaged 137.4 ± 18.5 and 92.8 ± 16.8 ng/ml, respectively, whereas the peak maternal and fetal plasma
concentrations of [2H10]DPMA were 28.7 ± 4.3 and 135.0 ± 20.1 ng/ml, respectively. The maternal-fetal
concentration differences for both forms of the metabolite were
significantly different from 0. The time at which the peak levels
occurred postinfusion was 18.0 ± 7.3 min for both labeled and
unlabeled DPMA in the ewe, whereas in the fetus the value was 87.0 ± 14.5 min. After the peak, the fetal metabolite levels declined much
more slowly than in the ewe. The elimination half-life of the
metabolite in the fetus and ewe (determined by simultaneous fitting of
the parent drug and metabolite data) was 15.2 ± 2.5 and 3.0 ± 0.2 hr, respectively. These values are significantly different. In
the two animals with functional UV catheters, the extraction ratio of
[2H10]DPMA across the fetal side of the
placenta averaged 0.06 ± 0.01. This value is not significantly
different from 0 but is different from the umbilical extraction ratio
for [2H10]DPHM given above. Finally, DPMA or
[2H10]DPMA metabolites were never detected in
amniotic or fetal lung fluid.
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Fetal and maternal renal elimination of DPHM, [2H10]DPHM, DPMA and [2H10]DPMA. The renal clearances of DPHM, [2H10]DPHM, DPMA and [2H10]DPMA in the ewe and fetus are given in table 3. DPMA and [2H10]DPMA were both present in adult urine during and after the infusion. In contrast, only very small quantities were detected in fetal urine. The cumulative excretion plot for DPHM and [2H10]DPHM in maternal and fetal urine clearly shows a plateau after the infusion (fig. 4A), whereas the metabolite appears to be near a plateau only at the end of the experimental protocol (fig. 4B). Thus, cumulative excretion of the metabolite may have been somewhat underestimated. The weight-corrected renal clearance of DPHM was ~200-fold less in adult sheep compared with fetal lambs, whereas the opposite situation existed for the metabolite (relative renal clearance ~50-fold greater in mother than in fetus). The contribution of renal DPHM clearance to maternal nonplacental clearance was 0.025 ± 0.011%, whereas in the fetus the contribution was 2.22 ± 0.42% (table 3). These values are significantly different. The percentage of total maternal DPHM and fetal [2H10]DPHM dose excreted as DPMA and [2H10]DPMA, respectively, averaged 0.95 ± 0.07% in the ewe and 0.014 ± 0.011% in the fetus. These values are also significantly different from each other.
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Study 3: Simultaneous Fetal UV and TV Administration
Figure 5 illustrates the
concentration-vs.-time plots for unlabeled and labeled forms
of DPHM and DPMA measured from samples obtained in our previous study
of fetal hepatic first-pass DPHM uptake after UV administration (Tonn
et al., 1996). Figure 5A shows the data from a bolus
experiment in which [2H10]DPHM was
administered via the UV, whereas figure 5B shows the data
from an infusion study in which unlabeled DPHM was infused via the umbilical route. In both experiments, there were no
consistent differences in the fetal arterial concentrations of DPHM and
[2H10]DPHM. In contrast, the plasma
concentration of the form of DPMA derived from the drug administered
via the UV was consistently higher than that derived from
drug given via the TV. Table 4 gives the FA plasma AUC values for labeled and unlabeled DPHM and DPMA.
The estimates of fetal first-pass hepatic extraction ratio based on
intact drug concentrations were obtained using equations 11 and 12, and
the mean value of 0.06 ± 0.06 is not significantly different
from 0, as reported previously (Tonn et al., 1996). In
contrast, the estimates of fetal hepatic extraction ratio obtained using the AUC values for DPMA and [2H10]DPMA
and equation 13 indicated significant drug uptake by the fetal liver.
The mean extraction ratio was 0.44 ± 0.05, and this was
significantly lower than the value of 0.71 ± 0.07 obtained above
in the paired maternal-fetal infusion protocol (table 2).
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Fetal and Maternal Plasma Protein Binding of DPMA
The time required to reach equilibrium for the determination of the binding of DPMA was 8 hr. No significant volume shifts were associated with this equilibrium time, and no nonspecific binding of DPMA to the equilibrium dialysis cell and the membrane could be detected. The metabolite was highly bound in both maternal and fetal plasma, with the percent bound averaging 99.4 ± 0.01% and 98.9 ± 0.07%, respectively. The free fraction in adult plasma (0.006 ± 0.002) was significantly less than that in fetal plasma (0.010 ± 0.001).
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Discussion |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Use of Stable Isotope-Labeled Compounds to Study Maternal-Fetal Drug Disposition
The current study appears to be the first in which a stable
isotope-labeled drug analog has been used to study maternal-fetal drug
disposition in pregnant sheep. The use of stable isotope-labeled compounds provides several advantages in studies of drug disposition during pregnancy, particularly in situations in which the simultaneous administration of the drug via two routes is to be used. As
noted in the introduction, our primary reason for using this
methodology in the current study was to eliminate the potential
confounding effects of fetal growth and maturation that occur over the
period between time-separated maternal and fetal drug infusions. This approach also reduces the overall duration of the experiment. This is
an important factor in studies involving chronically instrumented pregnant animals in which there is a finite time window available for
each preparation and, hence, shorter experiments allow for additional
studies to be conducted on the same animal. However, it is important
that the labeled and unlabeled forms of the drug be biologically
equivalent (Baillie, 1981). If this is not so, the labeled drug could
display different dispositional characteristics compared with the
unlabeled drug and thus be of limited use in pharmacokinetic studies
(Baillie, 1981). Consequently, it was first necessary to determine
whether such an "isotope effect" existed for
[2H10]DPHM in fetal sheep (study 1). The data
obtained on the concentrations of DPHM,
[2H10]DPHM, DPMA and
[2H10]DPMA during and after simultaneous
infusion of unlabeled and labeled parent drug at equivalent rates
via the TV suggest that the isotope effects with
[2H10]DPHM are negligible or absent in
pregnant sheep in terms of both the pharmacokinetics of the parent drug
and the formation and disposition of
[2H10]DPMA. The results are consistent with
our earlier data obtained in studies involving bolus drug
administration in fetal and nonpregnant sheep (Tonn et al.,
1996).
Study 2: Paired Maternal-Fetal Infusions
DPHM and [2H10]DPHM plasma concentrations
in the ewe and fetus.
The average total fetal plasma concentration
of DPHM achieved in the current experiments (i.e., DPHM + [2H10]DPHM = ~289 ng/ml) lies
between the two plasma concentrations achieved in the time-separated
maternal (~36 ng/ml) and fetal infusions (~450 ng/ml) in our
previous study (Yoo et al., 1993). In the ewe, the total
drug concentration in the current study (305 ng/ml) exceeds the levels
achieved in the previous maternal (212 ng/ml) and fetal (31 ng/ml)
infusions. Similar to our previous findings with simultaneous infusion
of unlabeled and labeled DPHM via the UV and TV (Tonn
et al., 1996), we did not find any evidence for preferential
delivery of maternally derived drug to the fetal brain and other upper
body structures. This is, however, the case with O2,
glucose and other nutrients that are present in higher concentrations
in the fetal ascending aorta compared with the descending aorta
(Charlton and Johengen, 1984). This feature is thought to be due to the
preferential distribution of umbilical venous blood to the upper body
(including the brain) (Edelstone and Rudolph, 1979). In contrast, in
the current study, the CA-FA concentration difference for DPHM
(administered to the ewe) was not significantly different from 0, whereas with [2H10]DPHM (infused
via the TV), there was a positive FA-CA difference (i.e., opposite to the situation with endogenous compounds).
As we previously discussed (Tonn et al., 1996), this
difference may be due to uptake of DPHM by the fetal lung, with a
resulting greater dilution of the drug with venous return in the left
heart (which primarily supplies the upper body) compared to the right
heart (which primarily supplies the lower body, see fig. 1).
Placental and nonplacental clearances of DPHM in fetal and maternal
sheep.
The maternal and fetal clearance values obtained for DPHM
in the current study are similar to those we previously determined (Yoo
et al., 1993). In particular, we confirmed that fetal
placental clearance of the drug is much higher than the maternal
placental clearance and that the weight-normalized fetal nonplacental
clearance is also greater than that in the ewe. In the current study,
CLfm was 5.4-fold higher than CLmf, whereas our
previous estimates were 3.7 times higher based on total drug
concentrations and 1.6 times higher based on free drug (Yoo et
al., 1993). The fetal transplacental and nonplacental clearance
values for DPHM are the highest of any drug examined in pregnant sheep;
this is also the case with the CLfm CLmf
difference. Given the overall agreement between the results of our two
studies, we conclude that this latter difference is not an artifactual
result of the time-separated maternal and fetal infusions in previous
studies that used the two-compartment open model.
). In a previous study in pregnant sheep, the fetal
placental clearance of acetaminophen estimated with the Fick method was not different from the clearance value calculated using the
two-compartment open model (Wang et al., 1986). However,
both CLfm (31 ml/min/kg) and CLfo (11 ml/min/kg) for acetaminophen are much lower than those for DPHM (table
1), so it was of interest to see whether the Fick and two-compartment
placental clearance rates for the latter compound would be similar.
Although the Fick estimates are lower than those obtained using the
two-compartment model, the difference was not great. Moreover, if there
was placental metabolism of DPHM, the Fick estimate of CLfm
should have been higher than the two-compartment value, whereas the
opposite situation was the case. Thus, for these two drugs with very
different physicochemical properties and clearance values, placental
drug metabolism does not appear to be of significance in terms of fetal
drug elimination in pregnant sheep.
Maternal and fetal plasma concentrations of DPMA and
[2H10]DPMA.
In humans, monkeys and dogs,
DPHM is thought to be metabolized via two sequential
N-demethylation steps followed by deamination to DPMA. This DPMA
metabolite and its conjugates are the major urinary metabolites of DPHM
in these species (Chang et al., 1974; Drach et
al., 1970; Drach and Howell, 1968; Glazko et al.,
1974). DPMA is also present in the urine and plasma of nonpregnant ewes after DPHM administration (Tonn et al., 1995). In the
present study, DPMA and [2H10]DPMA were
detected in both maternal and fetal plasma during and after the
simultaneous infusions of DPHM and [2H10]DPHM
to the ewe and fetus, respectively. The consistently higher
concentrations of the labeled metabolite in fetal plasma compared with
those in the mother during the infusion period provide strong evidence
for its formation in the fetus. The presence of DPMA in the fetus and
[2H10]DPMA in the ewe could be the result of
two processes: (1) placental transfer of DPHM to the fetus and
[2H10]DPHM to the ewe, with subsequent
formation of the unlabeled and labeled metabolites in fetal and
maternal compartments, respectively; and (2) fetal-to-maternal transfer
of [2H10]DPMA and maternal-to-fetal transfer
of DPMA. However, it seems unlikely that the latter process could be of
much importance because the minimal umbilical extraction ratio of
[2H10]DPMA (~0, see above) and the long
fetal elimination half-lives of the labeled and unlabeled metabolite
(~15 hr) suggest limited transfer across the ovine placenta. This is
perhaps due to a greater polarity of the metabolite compared with DPHM
and its high degree of plasma protein binding (~99%). However, the
larger maternal ratio for
AUC[2H10]DPMA/AUC[2H10]DPHM (0.96 ± 0.12) compared to AUCDPMA/AUCDPHM
(0.62 ± 0.07) suggests that at least a portion of the labeled
metabolite that is formed in the fetus is transferred to the mother.
The long half-life of the metabolite in the fetus also suggests that
the elimination pathways for this metabolite are not as well developed
in the fetus as they are in the ewe. We have, in fact, obtained recent data from studies involving fetal bolus administration of DPMA that
indicate that virtually all of the administered dose ultimately appears
in maternal urine over the ensuing 96 hr (Kumar et al., 1996). This confirms that both fetus and ewe have no detectable ability
to metabolize DPMA and that the metabolite can cross the sheep
placenta, albeit at a very slow rate. In other species, the
contribution of DPMA formation to overall DPHM elimination is high
(40-60%; Chang et al., 1974; Drach et al.,
1970; Drach and Howell, 1968; Glazko et al., 1974). However,
our recent studies in fetal and adult sheep suggest a much lower value
(~1%, Kumar et al., 1995, 1996).
Fetal and maternal renal elimination of DPHM,
[2H10]DPHM, DPMA and
[2H10]DPMA.
There appear to be
significant differences in the renal excretion of both DPHM and DPMA
between adult and fetal sheep. The renal clearance of DPHM in the
pregnant ewe (0.012 ± 0.005 ml/min/kg) is significantly less than
the reported GFR in adult sheep (~2.4 ml/min/kg; Hill and Lumbers,
1988). This suggests that a portion of the filtered and/or secreted
load of DPHM is reabsorbed in the renal proximal tubule. As a
consequence, the renal clearance of DPHM in maternal sheep contributes
<0.1% of the total body clearance. In contrast, the fetal renal
excretion of DPHM (~2.22 ± 0.42 ml/min/kg) exceeds reported
values for fetal GFR (~1 ml/min/kg; Hill and Lumbers, 1988). This
indicates fetal renal tubular secretion of DPHM in addition to
glomerular filtration of the drug. This finding is similar to the
results of previous studies on the renal excretion of various organic
cations in the late-gestational fetal lamb (cimetidine, ranitidine,
meperidine and tetraethylammonium), all of which have renal clearance
values that are greater than the GFR (Czuba et al., 1990;
Elbourne et al., 1990; Mihaly et al., 1983; Szeto
et al., 1979). In contrast to these amine compounds, the
fetal renal clearance of DPMA (0.013 ± 0.010 ml/min/kg) was not
significantly different from 0. There also is limited fetal renal
tubular secretion of para-aminohippurate, the glucuronide and sulfate conjugates of acetaminophen and morphine glucuronide (Elbourne et al., 1990; Olsen et al., 1988; Wang
et al., 1986). Also, we recently found the same phenomenon
with valproic acid5 and
indomethacin (Krishna et al., 1995).
). However, compounds in fetal blood may also reach
amniotic fluid via the intramembranous pathway (Gilbert
et al., 1995). The reason for the apparent lack of this
transport mechanism for DPMA may be its high degree of plasma protein
binding in fetal plasma.
Studies 2 and 3: Fetal Hepatic Uptake and Metabolism of DPHM
Evidence of fetal hepatic first-pass DPHM uptake from UV.
In a
previous study (Tonn et al., 1996), we examined the fetal
hepatic first-pass uptake of DPHM after UV drug administration after
both bolus and constant-rate intravenous infusions and found no
evidence for a first-pass effect. In contrast, a substantial (>90%)
hepatic presystemic elimination of the drug was observed with
mesenteric venous administration in adult sheep. However, the results
from the fetal experiments did not completely rule out the involvement
of fetal liver in DPHM metabolism/DPMA formation, and we recently
demonstrated formation of the DPMA metabolite when fetal hepatic
microsomal preparations are incubated with DPHM.6 The data from
study 2 on DPMA/DPHM (8.20 ± 1.62) and
[2H10]DPMA/[2H10]DPHM
AUC (2.24 ± 0.53) ratios in the fetus (table 2) indicate that
more of the maternally derived form of the drug (reaching the fetus
via the UV and hence undergoing a "partial" fetal
hepatic first-pass) is converted to the metabolite than is the form
administered directly to the fetus. These AUC ratios clearly
demonstrate that the fetal liver is involved in the metabolism and
nonplacental clearance of the drug. With equation 8 and the AUC ratios
from the current study, fetal hepatic first-pass extraction of DPHM present in UV blood averaged 0.71 ± 0.07. However, with the DPHM, [2H10]DPHM, DPMA and
[2H10]DPMA concentrations measured in samples
from our previous umbilical hepatic first-pass experiments (study 3)
and equation 13 (analogous to equation 8), a mean value of 0.44 ± 0.05 was obtained. We believe that the higher estimate of this
parameter obtained in the paired infusion study (study 2) is due to
maternal-to-fetal transfer of a portion of the maternally formed DPMA
to artifactually increase the fetal
AUCDPMA/AUCDPHM ratio. In the fetal hepatic first-pass study (study 3), both labeled and unlabeled DPHM were administered to the fetus, so that maternal-to-fetal transfer of intact
drug or metabolite was unlikely. Thus, the mean value of 0.44 for fetal
hepatic DPHM extraction estimated from direct fetal UV administration
is probably more accurate.
; Reuss and Rudolph, 1980). In contrast, ~50% of inferior vena
caval blood reaches the placenta (Edelstone and Rudolph, 1979; Reuss
and Rudolph, 1980). In addition, as was demonstrated in study 2 above,
~60% of the drug delivered to the placenta is extracted at this
site. Thus, after one pass through the fetal circulation, the average systemic availability of the drug (DPHM or
[2H10]DPHM) injected via the UV
will be ~50%. This is because on average, ~50% of the drug
injected via the UV is extracted in a single pass through
the circulation, calculated as the fraction removed via
hepatic first-pass extraction (~44%), plus the fraction extracted by
the placenta (~6%), for a total of ~50%. Similarly, after a
single pass through the fetal circulation, the systemic availability of
the drug administered at the inferior vena cava (TV) will be ~70%
because ~30% of the drug will be extracted at the placenta. In
addition to this factor, fetal circulatory transit times from UV to
placenta (~5.1 sec) and from inferior vena cava to placenta (~3.7
sec) are different (Power and Longo, 1975), whereas the transit time to
the placenta for the ~50% of the umbilical blood flow that passes
through the fetal liver is even longer (~9.8 sec; Power and Longo,
1975). Due to the above described factors, the form of drug
administered at the UV site likely experiences a "fetal hepatic
first-pass effect," whereas that administered at the TV site
experiences a "placental first-pass effect" (fig. 1). Thus, even
though a fetal hepatic first-pass DPHM uptake from UV blood was
present, the high placental extraction of drug administered via the TV may act to nullify the difference between
systemic concentrations (AUCs or Css) of the two forms of
the parent drug. This would result in minimal and inconsistent
differences in the systemic arterial levels and AUCs of the two forms
of drug and thus to an apparent lack of fetal hepatic DPHM elimination,
as was concluded in our previous study (Tonn et al., 1996).
However, if we assume that fetal hepatic DPHM elimination occurs
via its metabolism in the fetal liver and placental
elimination involves simple drug transfer to the maternal circulation,
there should be differences in the fetal plasma concentrations of the
DPHM metabolite (e.g., DPMA and
[2H10]DPMA) formed from the two forms of the
drug. Also, these differences are more likely to be maintained over
time because of the limited placental permeability of more polar and
highly protein bound DPMA (see above) in contrast to the parent drug,
which readily crosses placenta. In agreement with this, a consistent
concentration difference between the labeled and unlabeled forms of
DPMA in fetal arterial plasma was observed (study 3) that results from the hepatic first-pass uptake of umbilically administered drug and
subsequent formation of higher amounts of metabolite from this form of
the drug (fig. 5).
The data on fetal plasma DPMA and [2H10]DPMA
concentrations allowed an indirect estimation of the fetal hepatic
first-pass extraction of the parent drug after UV administration with
the use of equation 13. The estimate of 0.44 for fetal hepatic DPHM extraction is less than that found in adult sheep (0.93; Tonn et
al., 1996). However, ~50% of UV return bypasses the fetal liver via the ductus venosus (Holzman, 1984), and thus drug
present in this blood is not available for hepatic first-pass uptake. When the fetal hepatic extraction estimate is corrected for this, it is
similar to the adult value (0.88 vs. 0.92). Consequently, it
appears that the liver of the fetal lamb in late gestation is almost as
effective as the adult liver in metabolizing DPHM. Moreover, when the
"true" hepatic extraction estimate of 0.88 is multiplied by a
reported value for total hepatic blood flow in the fetal lamb (137 ml/min/kg fetal weight; Edelstone et al., 1978), the
resulting estimate of fetal hepatic clearance is ~120 ml/min/kg. This
comprises ~100% of CLfo (table 1), suggesting that the
fetal liver is the major organ responsible for fetal nonplacental
clearance of DPHM. Renal clearance of DPHM contributes only ~2% to
CLfo; previously, we found that fetal pulmonary extraction of DPHM contributes another 8% (Rurak et al., 1991). Thus,
combined average clearances of the liver, kidney and lung are ~10%
greater than our current estimate of CLfo, but given that
fetal hepatic extraction is estimated by an indirect method and that
the other data come from different studies, this difference is not too
great.
The metabolic fate of the DPHM taken up by the fetal liver remains to
be determined. As noted above, DPMA appears to play only a minor role
in the overall nonplacental elimination of the parent drug in both
fetal and adult sheep. We recently obtained evidence for the presence
of large amounts of an N-oxide metabolite of DPHM in adult and fetal
sheep plasma7 but
further studies are required to determine its quantitative importance
in the metabolism of drug.
Impact of fetal hepatic drug uptake on two-compartment model estimates of maternal and fetal clearances. The placental clearance values calculated using the two-compartment model are the "fundamental" clearances of the maternal-placental-fetal system and can be used to estimate the maximum possible rate of drug transfer across the placenta (under given conditions of blood flow and protein binding) assuming sink conditions on the other side. These clearance parameters are thus reflective of the true placental permeability of the drug in question. This is in contrast to the net rate of placental drug flux, which depends only on the rate of nonplacental drug elimination on the other side of placenta.
It is important at this point to realize that the proposed two-compartment system incorporates both maternal and fetal drug elimination. Hence, after both maternal and fetal drug administration, this system never reaches a state of equilibrium (defined as equal bidirectional drug fluxes and no net transfer of drug across the placenta). It does, however, reach a steady state in which the rate of drug flux across the placenta becomes equal to the rate of drug elimination from the other side of placenta. There could be two possible situations,
, Maternal DPHM; 
, maternal [2H10]DPHM; 
, fetal DPHM; 
, fetal
[2H10]DPHM.
