Departments of Pharmaceutics and Medicinal Chemistry, University of
Minnesota, College of Pharmacy, Minneapolis, Minnesota
Several in vitro and in situ approaches were used to determine
the dominant presystemic activation site for (
)-6-aminocarbovir, ()-carbocyclic
2',3'-didehydro-2',3'-dideoxy-6-deoxy-6-aminoguanosine (6AC) conversion in rats. The in vitro disappearance half-lives (mean ± S.D.) in the cytosolic fractions obtained from
homogenates of the intestine, liver, and intestinal contents were
0.4 ± 0.1 (n = 3), 12.2 ± 1.1 (n = 3), and 15.5 (n = 1) min,
respectively. An in situ vascularly perfused intestine-liver (IPIL)
study was then carried out (n = 6) to determine the
relative contribution of each presystemic organ to the overall
first-pass extraction of 6AC. The 6AC extraction ratios in the
intestine and liver in the IPIL were found to be 0.08 ± 0.02 and
0.11 ± 0.03, respectively. The intestinal extraction ratio was in
dramatic contrast to the in vitro results. It was postulated that
vascularly delivered 6AC had limited access to the metabolic site in
the intestine. A theoretical analysis suggested that the extent of
intestinal wall extraction of 6AC would be underestimated by the IPIL
and should be determined after oral dosing. To compare intestinal extraction ratio in the IPIL with that after an oral administration, in
situ intestinal lumen perfusions (n = 4) and
intraportal infusions (n = 3) of 6AC were conducted in
two groups of rats. The lumenally administered 6AC was extracted to a
much greater extent by the intestine as compared with the IPIL, which
presents 6AC to the intestine by the vascular route. The extraction
ratio was found to be 0.54 ± 0.06, which was significantly larger
than that obtained in the IPIL.
 |
Introduction |
()-Carbovir,
(()-carbocyclic 2',3'-didehydro-2',3'-dideoxyguanosine,
CBV)2 is a potent and
selective anti-HIV compound (Vince et al., 1988
) with a low oral
bioavailability and limited brain delivery (Huang et al., 1991; Wen et
al., 1995). When ()-6-aminocarbovir (()-carbocyclic 2',3'-didehydro-2',3'-dideoxy-6-deoxy-6-aminoguanosine, 6AC)) was
evaluated as a prodrug of CBV in rats, it exhibited superiority to the
parent drug in increasing systemic and central nervous system
exposure to CBV (Zimmerman et al., 1992; Wen et al., 1995). Much higher
CBV femoral blood concentrations were observed after an oral dose of
6AC as compared with i.v. administration of 6AC (Zimmerman et al.,
1992), indicating that 6AC was substantially converted to CBV in the
first-pass organs after dosing. Both the liver and intestine probably
contributed to the first-pass conversion of 6AC to CBV, but their
relative contributions to the first-pass activation of 6AC could not be
determined in these studies. Because 6AC is most likely metabolized to
CBV by adenosine deaminase (ADA) (Vince and Brownell, 1990), the
intestine may be the principal organ in the first-pass conversion of
6AC, as would be consistent with the tissue distribution of this enzyme
(Ho et al., 1980; Chinsky et al., 1990; Winston et al., 1992).
The objectives of the present studies were to investigate the relative
contributions of the liver and intestine to the first-pass conversion
of 6AC to CBV.
| |
Materials and Methods |
6AC and CBV were synthesized at the University of Minnesota
(Beers et al., 1990; Vince and Hua, 1990) and received as gifts from
Dr. Robert Vince. Trichloroacetic acid was purchased from Aldrich
Chemical Company (Milwaukee, WI), Dextran T-40 was purchased from
Pharmacia (Piscataway, NJ), and glucose was purchased from LyphoMed
Inc. (Rosemont, IL; dextrose injection, USP, 50%). All other chemicals
were reagent grade or better.
In Vitro Incubation of 6AC with Intestine, Liver, and Intestinal
Contents.
Initial studies were carried out with the cytosolic fraction from the
liver and intestine of rats. Three incubations each were carried out
with the intestine and liver. One incubation with intestinal contents
was conducted. For each incubation, the liver, intestine, and
intestinal contents from three male Sprague-Dawley rats (Bio-Labs, St.
Paul, MN) were harvested. The intestine was rinsed with 10 ml of
ice-cold phosphate-buffered saline (PBS) (pH 7.4) and the intestinal
contents were collected. The tissues were pooled and homogenized in PBS
with a Brinkmann Polytron (Westbury, NY). The organ weight to buffer
volume ratios were 1:10 for the intestine and 1:5 for the liver. The
homogenates were centrifuged at 10,000g at 4°C for 60 min.
The supernatant was then centrifuged at 100,000g at 4°C
for 60 min. Four milliliters of the final supernatant, which was the
cytosolic fraction, were preincubated for 5 min at 37°C, and 100 µl
6AC (400 µg/ml) was then added to start the incubation. Serial
samples of 100 µl each were taken in triplicate at specified
intervals up to 30, 120, and 360 min for the intestine, intestinal
contents, and liver, respectively. Samples were transferred into
ice-cooled microcentrifuge vials containing 400 µl of internal standard solution (0.8 µg/ml, carbocyclic 2',3'-dideoxyguanosine) and
10 µl of trichloroacetic acid (60%). Samples were immediately mixed
on a vortex mixer for 30 s. After centrifuging at
13,000g for 6 min in a Fisher (Pittsburgh, PA) model 235B
microcentrifuge, 25 µl of saturated NaHCO3 was added to
400 µl of the supernatant to neutralize the sample. The samples were
stored at 20°C until assay. 6AC was also incubated with PBS as a control.
Extraction of 6AC in the In Situ Vascularly Perfused
Intestine-Liver (IPIL).
Six male Sprague-Dawley rats (271.5 ± 26.2 g) were used. A
previously described surgical procedure (Hirayama et al., 1989; Xu et
al., 1989) was modified for use in the current study. The rats were
anesthetized with 50 mg/kg pentobarbital i.p. (Abbott Labs, North
Chicago, IL). A V-shaped incision was then made to expose the abdominal
cavity. The gastric artery, gastroduodenal artery, and splenic blood
vessels perfusing the stomach and spleen were ligated. A cannula of
Intramedic PE-20 polyethylene tubing (Clay Adams, Division of Becton
Dickinson and Co., Parsippany, NJ) with a beveled tip was inserted into
the bile duct and secured in place by ligation. The celiac artery and
the pyloric vein were ligated. A 20-gauge i.v. catheter placement unit
(Criticon Inc., Tampa, FL) was placed into the portal vein for portal
blood sampling and secured with Superglue. Immediately after the aorta
was tied off near the superior mesenteric artery, a cut was made in the superior mesenteric artery. A blunted 19-gauge × 11/2 inch
needle (Monoject, St. Louis, MO) was inserted into the artery. The
needle was secured with 3-0 surgical silk (Look Inc., Norwell, MA).
Perfusion into the superior mesenteric artery with blank perfusate was
immediately initiated at a flow rate of 2 to 3 ml/min. The thoracic
cavity was opened and a cut was made in the right atrium of the heart. The Teflon catheter from an i.v. placement unit was inserted into the
opening of the right atrium and secured in place. The catheter was
connected to Tygon tubing allowing the exit of perfusate from the
liver. The perfusion flow rate was then adjusted to approximately 10 ml/min.
The perfusate was a Krebs-Henseleit buffer (Pang, 1984) containing 300 mg/100 ml (v/v) glucose, 1% (v/v) bovine serum albumin (25% solution
in Tyrode's buffer; Sigma Chemical Co., St. Louis, MO), 3% (w/v)
Dextran T-40, and 20% (v/v) washed human red blood cells (American Red
Cross, St. Paul, MN). A perfusion apparatus (Perfuser Two/Ten; MX
International Inc., Aurora, CO) equipped with a peristaltic pump and an
oxygenator was used for the study. The viability of the perfused organs
was monitored by taking continuous pressure readings at the superior
mesenteric artery, by monitoring oxygen consumption in the portal and
hepatic veins, by monitoring L-aspartate 2-oxoglutarate
aminotransferase and lactate dehydrogenase in the hepatic vein and
portal vein perfusate, respectively, by monitoring the bile flow, and
by observing the gross appearance of the organs (Pang, 1984; Wen,
1995).
The organ extraction of 6AC in this preparation was examined at three
concentrations (0.4, 3.5, and 20 µg/ml). Each perfusion experiment
was divided into three periods. In period I (0-50 min), the organs
were perfused with a perfusate containing 6AC at one concentration.
Period I was followed by a washout period (period II, 50-70 min) with
blank perfusate. In period III (70-120 min), the organs were perfused
with a perfusate containing 6AC at a different concentration.
Preliminary studies showed that 6AC and CBV, converted from 6AC, were
not carried over from period I to period III. Because there were three
concentrations to be examined and each rat was to receive two different
concentrations, six treatment sequences were used. A total of 1600 ml
of perfusate was prepared for each experiment. A schematic
representation of the experimental setup is presented in Fig.
1. Perfusate samples of 300 µl each
were collected from the superior mesenteric artery, portal vein, and
hepatic vein at 7-min intervals from 20 to 48 min (period I) and from
90 to 118 min (period III). Aliquots of exactly 200 µl of sample were
pipetted into plastic microcentrifuge vials containing 800 µl of
internal standard solution (0.8 µg/ml) and 20 µl of
2'-deoxycoformycin (DCF) (pentostatin; Parke-Davis Pharmaceuticals, Ann
Arbor, MI) solution (1 mg/ml). DCF is an ADA inhibitor that was added
to prevent the in vitro conversion of 6AC to CBV. After mixing, samples
were placed on dry ice for the remainder of the experiment and then
frozen at 70°C until assay.
Extraction of 6AC in Intestine during Intestinal Lumen Perfusion
Theory.
The IPIL studies described above showed that the intestine and liver
had similar abilities to extract 6AC. This was in marked contrast to
the data generated from the in vitro homogenate incubations in which
the intestinal tissue was much more active in converting 6AC than was
the liver tissue (see Results). This suggested that the
intestinal extraction of 6AC might not be a perfusion rate-limited process. Movement of 6AC from the blood to the enzyme site may play an
important role in the extraction process, especially because there is
evidence that ADA, the enzyme catalyzing the conversion, is located
near the brush border membrane of the intestine (Holt et al., 1985;
Chinsky et al., 1990). Assuming that the blood flow is in rapid
equilibrium with the "serosal" space, and the ADA is located
distally in a "mucosal" space, a typical 6AC molecule would have a
different probability of being converted to CBV when it was supplied by
the blood stream perfusing the intestine than when it was supplied to
the apical side of the intestinal mucosa (Fig.
2). Therefore, the extraction ratio of
6AC (E) obtained from the IPIL preparation might not be an accurate
representation of the extraction ratio (Epo) when 6AC was
administered to the intestinal lumen. A theoretical analysis based on
the model described in Fig. 2 was performed to elucidate the
relationship between E and Epo. Because ADA is localized
near the mucosal side of the cell, the model in Fig. 2 shows no
conversion of 6AC to CBV in the serosal space of the intestinal wall.
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Fig. 2.
Model for intestinal extraction of 6AC. In
the model pictured, Clfsys is the abbreviation for
CLsysf (the formation clearance to
CBV in the systemic compartment) and Clfgw is the abbreviation for
CLgwf (the formation clearance to
CBV in the mucosal compartment).
|
|
The following equations were obtained (see Appendix 1 for
the detailed derivation):
|
(1)
|
|
(2)
|
where: Qpv = portal vein blood flow,
CLgwf = intrinsic formation clearance of 6AC to
CBV in the mucosal compartment of the intestinal wall, and
CLgw,dif = diffusional clearance of 6AC in the intestinal
wall (assumed to be a passive process and equal in both directions).
From equations 1 and 2, the relation of E to Epo can be
obtained:
|
(3)
|
Equation 3 indicates that the extraction ratio obtained from
IPIL (E) would be an underestimate of the extraction ratio of a drug
administered orally (Epo) if its metabolism was rate
limited by its access to the metabolic site. The rate process for the movement to the metabolic site is designated CLdif,gw.
Based on the discrepancy in the data generated from the homogenate and IPIL studies, it was hypothesized that 6AC delivered to the intestine by the vasculature was limited in its access to ADA. The following experiment was designed to provide in vivo evidence for this hypothesis.
Modified Multiple Site of Administration Technique.
A total of seven male Sprague-Dawley rats (264 ± 15 g;
Bio-Labs) was divided into two groups. The experimental setup is
described in Fig. 3. Four rats received a
lumenal perfusion of 6AC through an intestinal segment. Three rats
received an infusion of 6AC via the portal vein. The rats were under
pentobarbital anesthesia for the entire duration of the perfusion or
infusion. For the rats in the perfusion group, a 40-cm segment of the
small intestine starting from the ligament of Treitz was isolated with
the vasculature kept intact. Both ends of the segment were connected to
custom-made glass cannuli. The contents in the intestinal segment were
initially flushed with normal saline. The duodenal end of the segment
was connected to a 50-ml plastic syringe. The segment was perfused with
6AC in HEPES buffer for 100 min at a rate of approximately 80 µg/min
with a Harvard microliter syringe pump. The volumetric flow rate was
0.21 ml/min. Perfusate was collected from the distal cannula in 10-min
fractions. In the rats receiving the portal vein infusion, the portal
vein was catheterized with an i.v. catheter placement unit, which was
connected to a 12-ml plastic syringe. 6AC in normal saline was infused
into the portal vein for 100 min at a rate of approximately 28 µg/min
with a Harvard microliter syringe pump. An ileac vein catheter
(Silastic tubing connected to PE-50 tubing) was implanted for blood
sampling for both routes of administration. Four to five blood samples
of 150 µl each were withdrawn from the rats starting approximately 40 min after the initiation of the perfusion or infusion. Blood samples
were first placed into heparinized Vacutainers (Becton Dickinson,
Franklin Lakes, NJ) and the tubes were gently inverted five times.
Aliquots of 100 µl of the blood samples were pipetted into
microcentrifuge vials, to which 400 µl of internal standard solution
(0.8 µg/ml) and 10 µl of DCF solution (1 mg/ml) had previously been
added. After vortexing, blood samples were placed on dry ice for the remainder of the experiment and then kept at 70°C until assay.
Data Analysis.
Disappearance Half-Life of 6AC in Tissue Incubations.
The disappearance rate constant (k) of 6AC in each tissue
incubation was obtained by linear regression of the logarithmic concentration-time data. The disappearance half-life
(T1/2) was calculated from this first-order rate constant.
Intestine and Liver Extraction Ratio of 6AC in the IPIL.
The instantaneous organ extraction ratio (E) of 6AC was calculated
using eq. 4:
|
(4)
|
where Cin and Cout are the 6AC
concentrations in the influent and effluent blood flows, respectively.
For the intestine, Cin was the concentration of 6AC
entering the superior mesenteric artery and Cout was the
concentration of 6AC in the hepatic portal vein. For the liver,
Cin was the concentration of 6AC in the portal vein and
Cout was the concentration of 6AC in the hepatic vein.
Intestine Extraction Ratio of 6AC via Intestinal Lumen Perfusion
(Epo).
Although eq. 2 is a theoretical construct that suggests the
physiological variables that make up Epo, it was necessary
to derive an expression for Epo that could be calculated
based on the data generated by experiments. To obtain the extraction
ratio of 6AC in the intestine after an intestinal lumen administration of 6AC, an intraportal administration of 6AC was also required. The
extraction ratio could then be derived based on the mass balance principle at steady state (Appendix 2).
Fgw6AC, the fraction of 6AC surviving the
intestinal wall metabolism, is calculated as a function of steady-state
concentration ratios (CR) of CBV to 6AC after oral (CRperf)
and after portal infusion (CRinf):
|
(5)
|
Epo is then obtained from eq. 6:
|
(6)
|
Figure 3 describes the experimental system.
In these anesthetized animals, 6AC exhibited a decrease in systemic
clearance compared with a previous in vivo study (Zimmerman et al.,
1992) in awake animals. Because CBV systemic clearance was not
separately determined in this study, Fmsys was calculated (via eq. A19) by assuming that anesthesia reduced the CBV systemic clearance by the same percentage as it did the 6AC systemic clearance.
Analytical Methods.
Both 6AC and CBV in all matrices were analyzed by validated solid-phase
extraction procedures and high-performance liquid chromatography assays
(Zimmerman et al., 1992; Wen, 1995). Blood perfusate and whole-blood
samples underwent two cycles of freezing and thawing to lyse the red
blood cells. They were then centrifuged and the supernatant was applied
to C18 solid-phase extraction columns. The homogenates and
intestinal content samples were centrifuged and the supernatant applied
to the solid-phase extraction column in preparation for quantitation by
high-performance liquid chromatography.
| |
Results |
In Vitro Tissue Homogenate Incubations.
Figure 4 shows the 6AC and CBV
concentration-time profiles in incubations with the intestinal
homogenate, liver homogenate, and intestinal contents. The incubation
with the liver homogenate was actually conducted over 360 min, but 6AC
and CBV profiles are only shown for the first 120 min for easier
comparison with the intestinal incubations. Incubations in all three
media achieved complete conversion of 6AC to CBV, judging by mass
balance.
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Fig. 4.
Mean 6AC ( ) and CBV ( )
concentration-time profiles (n = 3) in intestinal homogenate
incubations (A), intestinal content incubations (B) and liver
homogenate incubations (C).
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|
Table 1 summarizes the 6AC disappearance
half-lives, corrected for the dilution before homogenization. The
intestine appears to be the most active tissue in converting 6AC to
CBV. 6AC disappears from the intestinal homogenate approximately 30 times as fast as from the liver homogenate.
In Situ IPIL.
Figure 5 shows representative 6AC and CBV
concentration-time profiles from an IPIL experiment. In this case, the
initial 6AC concentration (20 µg/ml) was later switched to a lower
concentration (3.5 µg/ml). No carryover of either 6AC or CBV was
observed in preliminary studies because of the appropriate wash-out
period. The shallow slope of 6AC profiles in the perfusate (superior
mesenteric artery) indicates that there was a slow conversion of 6AC to
CBV in the perfusate itself. This conversion proved to be insignificant relative to the overall conversion of 6AC taking place in the perfused
organs. Nevertheless, the instantaneous extraction ratio of 6AC in an
organ was calculated at each time point using eq. 4.
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Fig. 5.
6AC and CBV concentration-time profiles in
a representative IPIL experiment. CBV and 6AC concentrations at the
superior mesenteric artery (sm), the portal vein (p) and the hepatic
vein (h) are depicted. The starting reservoir concentration of 6AC in
phase I was 20 µg/ml and was 3.5 µg/ml in phase III.
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Table 2 contains the average of the
instantaneous 6AC extraction ratios in the intestine and liver of each
rat in the IPIL study. There was no significant effect of 6AC
concentration, perfusion period, or treatment order on the extraction
ratio in either organ (analysis of variance). The mean extraction
ratios of 6AC in the intestine and liver were approximately 0.08 ± 0.02 and 0.11 ± 0.03, respectively. The results are in marked
contrast to the incubation studies that indicated that the intestine
should have been much more active in converting 6AC to CBV.
Viability of the perfused organs was monitored frequently by a variety
of measurements as described in Materials and Methods. Except for the blood pressure at the superior mesenteric artery, which
increased gradually as the experiment went on, other viability measurements such as L-aspartate 2-oxoglutarate
aminotransferase and lactate dehydrogenase levels, oxygen consumption,
and bile flow rate all appeared to be normal throughout the time of
perfusion (Wen, 1995).
Intestinal Lumen Perfusion and Intraportal Infusion.
Figure 6 shows the mean 6AC and CBV
concentration-time profiles after intraportal infusion and intestinal
lumen perfusion of 6AC, respectively. Steady state for both 6AC and CBV
was apparently achieved quickly. The steady-state concentration used in
the parameter computation was the average of those concentrations
considered to be at steady state by observation. The ratio of CBV
concentration to 6AC concentration was much greater after intestinal
lumen perfusion than after intraportal infusion. This indicates a more
substantial conversion of 6AC to CBV in the intestine after intestinal
lumen perfusion of 6AC.
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Fig. 6.
Blood concentration profiles (mean ± S.D.) after intraportal infusions (A, n = 3) and intestinal lumen
perfusions (B, n = 4).
|
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Table 3 summarizes the results from this
study. The extraction ratio (Epo) was calculated to be
0.54 ± 0.06, significantly larger than the extraction ratio (E)
of 0.08 ± 0.02 in the IPIL study.
| |
Discussion |
The carbocyclic nucleosides, represented by the prototype
molecule, CBV, are novel reverse transcriptase inhibitors with
significant activity against HIV (Vince et al., 1988). An analog of
CBV, abacavir, is currently in clinical trials (Faletto et al., 1997).
The present work continued the preclinical investigations of another
CBV analog, 6AC, and the mechanism of its enhanced systemic delivery of
CBV after oral dosing. ADA, the enzyme responsible for the conversion
of 6AC to CBV, is localized in the presystemic organs, with the
intestine having significantly greater activity than the liver (Ho et
al., 1980; Chinsky et al., 1990). For 6AC, the intestine should be the
primary organ where most of the first-pass effect takes place after an
oral dose. Indeed, the disappearance half-lives of 6AC in the in vitro
incubation studies were in accord with the relative tissue distribution
of ADA. Homogenate incubations are often used as a means for in vitro
prediction of in vivo metabolism. Obviously, tissue homogenates differ
from the tissue itself by the lack of intact cellular membranes. Less
obviously, the compartmentalization of the enzymatic environment in the
living tissue is lost in the homogenate. Nevertheless, good in
vitro-in vivo correlations have been found for a large number of
compounds (Houston, 1994).
However, the extraction of 6AC in the intestine in the IPIL was
drastically different from what was predicted from the in vitro
incubation results. The intestinal homogenate was much more active in
converting 6AC to CBV in vitro than was the liver homogenate. In
contrast, in the IPIL the intestine and liver were about equal in their
apparent ability to extract 6AC. This suggested that the intestinal
extraction of vascularly delivered 6AC was limited for some reason. One
plausible explanation was that vascularly delivered 6AC might have had
restricted access to the drug-metabolizing enzymes. To test this
hypothesis, the extraction ratio of orally administered 6AC
(Epo) was determined with the use of the lumenal perfusion
technique, and a significantly higher value was obtained, indicating
that the IPIL underestimated the intestinal extraction of 6AC. In this
calculation, it was assumed that both 6AC and CBV clearances decreased
to a similar extent as a result of anesthesia. Ideally, simultaneous
estimation of CBV and 6AC clearance should have been obtained. However,
this was not done for a variety of reasons, including the lack of
availability of radiolabeled CBV. On the other hand, Fmsys
calculated with this approach (Table 3) approximated the previous value
of 0.48 ± 0.14 reported in conscious rats (Zimmerman et al.,
1992).
A model was then developed to illustrate the relationship between the
extraction ratio of vascularly delivered 6AC in the IPIL (E) and the
extraction ratio of orally absorbed 6AC (Epo). It is clear
from eq. 3 that the interrelationship of E and Epo is
determined by the access of 6AC molecules to the enzyme site (CLgw,dif) and the portal blood flow (Qpv).
When the diffusional process is much faster than the convective portal
blood flow, the value of E will approach Epo. The
intestinal wall extraction determined in an IPIL experiment would then
be an accurate estimate of the extraction ratio after an oral dose.
The ability to diffuse across a membrane or through the cytoplasm to
the enzyme site will depend on the physicochemical characteristics of
the drug as well as the organ distribution of the enzyme. If the
diffusional process for 6AC is slow compared with the convective perfusate flow, many prodrug molecules will be carried through the
extracting organ by the perfusate flow without having had the
opportunity to diffuse to the metabolic site. Although there may be
large amounts of metabolizing enzyme in the intestine, as suggested by
the incubation results, there is a localization of enzyme activity that
limits its ability to activate vascularly delivered 6AC. In the present
case, CLgw,dif was estimated for the IPIL experiment with
eq. 3 and the data in Tables 2 and 3. The CLgw,dif was
calculated to be 1.74 ml/min, considerably lower than the
Qpv used in the IPIL preparation (10 ml/min). This
indicates that the intestinal wall extraction of a compound such as 6AC would be underestimated by the IPIL, and an accurate estimation of the
extent of extraction could only be determined by oral dosing. Additional validation of this model could be done by carrying out
perfusion studies at flow rates closer to the estimated
CLgw,dif.
The process of serosal 6AC moving to the enzyme site has been described
here as a diffusional clearance, a concept long-recognized in the organ
distribution of certain drugs and metabolites (Dedrick et al., 1975;
Sato et al., 1986; Brouwer and Jones, 1990; Pang et al., 1984; Gwilt et
al., 1988; Schwab et al., 1990). This, however, implies a rate-limiting
membrane, which may be unnecessarily restrictive. Lack of access may
also be caused by the compartmentalization of the metabolizing enzymes
(Sato et al., 1986), i.e., the intestinal cell is not
"well-stirred" (Rowland et al., 1973). If the enzyme is located
near the mucosal side of the cell, as is the case for ADA (Holt et al.,
1985; Chinsky et al., 1990), 6AC molecules being absorbed from the
lumen will have greater contact time in the drug-metabolizing
compartment than will 6AC molecules being swept through the gut wall by
the blood flow.
An alternative interpretation of the present findings is that the
superior mesenteric arterial flow is actually fractionated into flows
separately perfusing the metabolically active mucosa and other
metabolically inactive subregions of the intestine (Klippert and
Noordhoek, 1983). Drug delivered by the oral route would by necessity
be carried into the portal venous flow by the mucosal blood. Drug
delivered systemically would be exposed to the metabolically active
mucosa blood in only a fraction of the total mesenteric blood flow.
This fractionation of blood flow could thus lead to the described
discrepancy in the intestinal extraction ratio of drug delivered by the
two routes. This explanation also supports the contention that the
intestine is not a well-stirred organ.
Conclusions.
Several approaches, both theoretical and experimental, have been used
to determine the dominant presystemic site for 6AC conversion. The in
vitro homogenate incubations suggested that the intestine was the most
active organ in converting 6AC to CBV. However, the in situ perfused
intestine-liver appeared to be limited in its ability to predict the
intestinal wall extraction of 6AC. A theoretical analysis pointed out
that the extent of intestinal wall extraction of 6AC should be
determined after an oral dose. Indeed, after intestinal lumen
perfusion, 6AC was extracted to a much greater extent in the intestine
as compared with the IPIL. In other words, the intestine cannot be
considered to be well-stirred with respect to the metabolism of 6AC.
The positive aspect of a substantial first-pass conversion of prodrugs
is that the systemic exposure to the active drug is increased, which is
probably the goal for most oral prodrugs. On the other hand, if
subsequent delivery to a targeted tissue and/or organ is desired, e.g.,
the brain, then such a first-pass effect might not be viewed favorably.
In the case of 6AC, because the first-pass conversion of 6AC primarily
takes place in the intestine, quenching of the intestinal activation of
6AC by orally administering ADA inhibitors may result in an increase in
6AC bioavailability, which may in turn improve brain exposure to CBV (Wen et al., 1995). Results of such inhibition studies will be presented in the second article of this series.
We acknowledge the gift of CBV and 6AC from Drs. Robert Vince and
Phuong T. Pham, Department of Medicinal Chemistry, University of
Minnesota. We also acknowledge the helpful comments of the reviewers of
the original manuscript.
This work was partially supported by Public Health Service
Grant R01-AI28236 and the University of Minnesota International Student
Work Opportunities Program.
At steady state during an intraportal infusion, the mass balance
equations are as follows:
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)-6-Aminocarbovir in Rats. I. Prodrug Activation May Be Limited by Access to Enzyme
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Abstract
Introduction
