Kinetic Analysis of the Transport of Salicylic Acid, a Nonsteroidal Anti-inflammatory Drug, across Human Placenta

Kyohei Shintaku, Yuka Arima, Yukihiko Dan, Tsutomu Takeda, Kentaro Kogushi, Masayuki Tsujimoto, Hideaki Nagata, Shoji Satoh, Kiyomi Tsukimori, Hitoo Nakano, Satoko Hori, Hisakazu Ohtani, and Yasufumi Sawada

Department of Medico-Pharmaceutical Sciences, Graduate School of Pharmaceutical Sciences (K.S., Y.A., Y.D., T.T., K.K., M.T.), and Department of Reproduction and Gynecology, Graduate School of Medical Sciences (H.Nag., S.S., K.T., H.Nak.), Kyushu University, Fukuoka, Japan; and Department of Drug Informatics, Graduate School of Pharmaceutical Sciences, the University of Tokyo, Tokyo, Japan (S.H., H.O., Y.S.)

(Received September 19, 2006; accepted February 14, 2007)

Abstract

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Abstract
Materials and Methods
Results
Discussion
References

The aim of this study was to develop a pharmacokinetic modelto describe the transplacental transfer of drugs, based on thehuman placental perfusion study. The maternal and fetal sidesof human placentas were perfused with salicylic acid togetherwith antipyrine, a passive diffusion marker. The drug concentrationin the placental tissue was determined at the end of perfusion.A compartment model consisting of maternal space, fetal intravascularspace, and placental tissue was fitted to the observed concentrationprofiles of salicylic acid in the maternal and fetal effluents.The developed model could adequately explain the concentrationprofiles of salicylic acid in the effluents with influx clearancesfrom maternal and fetal perfusates to placental tissue of 0.0407and 0.0813 ml/min/g cotyledon and efflux rate constants fromplacental tissue to maternal and fetal perfusates (k₂ and k₃)of 0.0238 and 0.176 min^–1, respectively. The kineticsof antipyrine was adequately described by assuming rapid equilibriumbetween fetal perfusate and placental tissue compartments. Theinflux plasma clearance from the maternal side (K''₁) in humanswas estimated by taking into account the protein binding. TheK''₁/k₂ value of salicylic acid was 1.07 ml/g cotyledon andwas larger than that of antipyrine (0.642 ml/g cotyledon). Weevaluated the transplacental transfer kinetics of salicylicacid by human placental perfusion study with various perfusionprotocols. Based on the data obtained, we developed a pharmacokineticmodel, which should enable us to estimate the influx profileof drugs into umbilical arterial blood from the maternal plasmaconcentration profile.

Exchange of materials between mother and fetus occurs acrossthe placenta (Robertson and Karp, 1976

), where fetal blood perfusesthe villi and maternal blood fills the interstitial space. Theblood-placental barrier consists of trophoblasts, which facethe interstitial space, and fetal capillary endothelium (Stulc,1989

). To estimate the distribution of a drug into the fetus,it is essential to investigate the transplacental transfer process.

Human placental perfusion, first designed by Schneider et al.(1972), is a useful technique to investigate drug transfer fromthe maternal to the fetal circulation in humans, because theinflux and efflux profiles of the drug can be directly observed.In vivo distribution studies with pregnant animals cannot providesuch information and also suffer from the problem of interspeciesdifferences. The placental perfusion technique is also preferableto in vitro methods using cultured human cell lines, such asBeWo or Jar, or membrane vesicles prepared from human placenta(Martel and Keating, 2003; Manley et al., 2005), because physiologicalmetabolism is quite well retained (Nanovskaya et al., 2002).However, many studies using human placental perfusion have providedonly simple information, i.e., the ratio of drug concentrationin fetal effluent to that in maternal effluent (Heikkinen etal., 2000; Nekhayeva et al., 2005). No studies have been conductedto analyze the kinetic features of drug transfer among maternalperfusate, placental tissue, and fetal perfusate by using thehuman placental perfusion technique.

Salicylic acid is widely used as an antipyretic and analgesic.However, intake of salicylic acid at pregnancy is reported tobe negatively correlated with fertility and body weight of newborns(Turner and Collins, 1975). When given at full-term pregnancy,salicylic acid readily permeates into fetal blood, inhibitingthe synthesis of prostaglandins and inducing constriction ofthe ductus arteriosus, which leads to pulmonary hypertensionin the newborn (Perkin et al., 1980). Therefore, it is worthwhileto investigate in detail the kinetics of the transfer of salicylicacid from mother to fetus.

The aims of this study are to develop a pharmacokinetic modelto describe the transfer kinetics of drugs among maternal blood,placental tissue, and fetal blood, and to analyze quantitativelythe transfer properties of salicylic acid across the blood-placentalbarriers by applying the developed model.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Materials. Human full-term placentas were obtained from gravidaeafter normal vaginal or cesarean delivery. The study protocolwas approved by the Ethical Committee of the Faculty of Medicine,Kyushu University, and written informed consent was providedby the gravidae. Salicylic acid, antipyrine, phenobarbital,4-aminoantipyrine, heparin, and human serum albumin were purchasedfrom Nacalai Tesque (Kyoto, Japan). All other reagents usedwere of the highest grade commercially available.

Solutions. The perfusate (Krebs-Ringer-bicarbonate buffer) consistedof 118 mM NaCl, 4.7 mM KCl, 1.3 mM MgSO₄, 24.2 mM NaHCO₃, 2.5mM CaCl₂, D-glucose (1.0 g/l), heparin (12,500 IU/l), dextran(1.0 g/l), and human serum albumin (2.0 g/l).

Salicylic acid (test drug) and antipyrine (passive diffusionmarker) were each dissolved in the perfusate to give concentrationsof 8 µg/ml and 50 µg/ml, respectively. The pH wasadjusted to 7.4 with 1 M HCl. The maternal and fetal perfusateswere aerated with 95% O₂/5% CO₂ and 95% N₂/5% CO₂, respectively,and warmed to 37°C.

Drug Transfer from Maternal to Fetal Side (Protocol I). In vitrohuman placental perfusion was carried out based on the methodreported by Schneider et al. (1972). A cotyledon (4–6cm in diameter) was chosen from a placenta obtained after vaginalor cesarean delivery. The fetal artery of the cotyledon wascannulated, ligated, and perfused with drug-free perfusate ata rate of 3 ml/min for 30 min by using a peristaltic pump (microtube pump; EYELA, Tokyo, Japan). Then, while perfusion was continued,the cotyledon was dissected from the placenta and mounted ona plastic chamber with the maternal side up. Three needles (18gauge) were inserted from the maternal side to a depth of 7mm and maternal perfusate was perfused via the needles at arate of 15 ml/min for 30 min to stabilize the preparation. Throughoutthe experiment, the fetal perfusion pressure was monitored witha personal computer (PC7200/900, Macintosh; Apple Computer,Cupertino, CA) equipped with a pressure transducer (Single TransducerSet; Nihon Kohden, Tokyo, Japan), an A/D converter (Power Lab/200;Nihon Kohden), and an amplifier (RMP-6004M; Nihon Kohden). Bothsalicylic acid and antipyrine were dissolved in maternal perfusateand perfused from the maternal side. Maternal and fetal effluentswere sampled for 60 min. Before sampling, the effluent in thematernal chamber was stirred to ensure thorough mixing. In allthe perfusion protocols, perfused cotyledon was weighed andalso sampled just after the last sampling of effluent to determinethe tissue concentrations of drugs. All the samples were storedat –20°C until analysis.

Drug Efflux from the Placenta (Protocol Ia). After perfusionof the cotyledon with drug-containing perfusate from the maternalside for 62 min as in protocol I, the maternal perfusate waschanged to a drug-free perfusate and the effluents from bothmaternal and fetal sides were further sampled for 3 min.

Initial Distribution of Drugs into Placental Tissue (ProtocolIb). After a 30-min stabilization as in protocol I, the maternaland fetal sides were perfused with drug-containing buffer anddrug-free buffer, respectively, for 5 min to obtain the placentalsample at 5 min.

Drug Transfer from Fetal to Maternal Side (Protocol II). Aftera 30-min stabilization as in protocol I, the fetal and maternalsides were perfused with drug-containing buffer and drug-freebuffer, respectively, for 52 min.

Determination of Antipyrine Concentration in Effluents. Concentrationsof antipyrine in effluents were determined by an HPLC-UV method.A sample (500 µl) was spiked with 500 µl of internalstandard solution (50 µg/ml 4-aminoantipyrine in ethanol),shaken for 1 min, and centrifuged at 15,500g for 10 min at 4°C.The supernatant was dried under a gentle stream of nitrogengas and the residue was dissolved in 1 ml of mobile phase (0.02M phosphate buffer, pH 6.0/methanol, 70:30 v/v). An aliquotof 20 µl of the solution was subjected to HPLC. The determinationlimit was 0.1 µg/ml.

Determination of Salicylic Acid Concentration in Effluents.Concentrations of salicylic acid in effluents were determinedby an HPLC-UV method. A sample (500 µl) was spiked with500 µl of internal standard solution (50 µg/ml phenobarbitalin water), 5 ml of chloroform, and 50 µl of 1 M HCl, mixedfor 1 min, and spun at 740g for 10 min at 4°C. The organiclayer (4 ml) was transferred to a glass tube and evaporatedinto dryness under a gentle stream of nitrogen. The residuewas dissolved in 200 µl of mobile phase (0.04 MKH₂PO₄,pH 2.0/H₂O/acetonitrile, 40:35:25 v/v) and an 80-µl aliquotwas subjected to HPLC. The determination limit was 0.1 µg/ml.

Determination of Drugs in Placental Tissue. Placental concentrationsof drugs were determined by the HPLC-UV method. A weighed placentalsection was cut into small pieces with scissors, added to 2volumes of water, and homogenized with a blender (Physcotron;Microtech Nichion, Chiba, Japan) and a Teflon homogenizer (MiniD.C. stirrer, EYELA). An aliquot of 3 ml of the homogenate wasspiked with 50 µl of 1 M HCl, 5 ml of chloroform, and10 µl of internal standard solution (50 µg/ml 4-aminoantipyrinein ethanol for antipyrine and 50 µg/ml phenobarbital inwater for salicylic acid), mixed for 1 min, and spun at 740gfor 20 min at 4°C. The organic layer (3 ml) was transferredto a glass tube, evaporated to dryness under a gentle nitrogenstream and dissolved in 1 ml of the mobile phase. The supernatant(500 µl) was spun at 15,500g for 10 min and a 20-µlaliquot was subjected to HPLC.

HPLC Apparatus. The HPLC system consisted of a pump (LC-10AD;Shimadzu Co., Kyoto, Japan), a UV-visible detector (SPD-10AV;Shimadzu), and an integrator (CR-6A Chromatopac; Shimadzu).A reversed-phase column (Cosmosil 5C18, 4.6 mm x 150 mm, 5 µm;Nacalai Tesque) was used for separation at ambient temperature.The mobile phases described above were pumped at a rate of 1.0ml/min. The detection wavelength was set at 250 nm or 235 nmfor the determination of antipyrine or salicylic acid, respectively.

Evaluation of Transplacental Permeability. The value of TPT_ss(ratio of the rate of amount transferred across the placentato that infused in the steady state) was calculated as the ratioof the amount transferred across the placenta to that infusedat the steady state in protocol I or Ia by using eq. 1 (Heikkinenet al., 2000).

Formula (1)
whereCf_ss, C_in, Q_f, and Q_m represent the mean drug concentrationin the fetal effluent samples at steady state, the drug concentrationin the maternal perfusate, and the fetal and maternal flow rates(3 and 15 ml/min), respectively.

Outline of Pharmacokinetic Analysis (Fig. 1). The experimentaldesign was as follows. One of the above protocols was appliedto each placenta to obtain one set of concentration-time profilesof antipyrine and salicylic acid in maternal and fetal effluents.Then, all the time profiles for each compound were pooled, andthe appropriate pharmacokinetic model described below was simultaneouslyfitted to the collective data to obtain pharmacokinetic parameters.

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FIG. 1. Schematic representation of the experimental design. A set of concentration-time profiles of antipyrine and salicylic acid in maternal and fetal effluents was obtained from one placenta. Then, all the time profiles of each compound in the four experimental protocols were pooled. Finally, the appropriate pharmacokinetic model was simultaneously fitted to the collective data to obtain pharmacokinetic parameters. See the text for details of the pharmacokinetic models.

Model Analysis for Antipyrine (Fig. 2). A pharmacokinetic modelconsisting of two placental compartments (i.e., maternal compartmentand placental tissue compartment) and a dead volume compartmentfor the maternal reservoir, where the three needles were attached,was used to evaluate the transplacental transfer kinetics ofantipyrine. The maternal compartment consists of the interstitialspace and the maternal chamber that receives the maternal effluent.The volume of the maternal compartment, V_m, was assumed to be23 ml. The influx rate constant from the dead volume compartmentinto the maternal compartment, k_a, was determined to be 1.02min^–1 by analyzing the time profile of antipyrine in theeffluent from the three needles after changing the influx solutionfrom drug-free to drug-containing perfusate.

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FIG. 2. Pharmacokinetic models of antipyrine transfer across the placenta observed with a human placental perfusion method. C_in, drug concentration in perfusate (50 µg/ml); C_m, drug concentration in maternal compartment (µg/ml); C, drug concentration in fetal intravascular compartment (µg/ml); X_p, amount of drug in placental compartment (µg/g cotyledon); k_a, first-order influx rate constant (1.02 min^–1); K₁, influx clearance (ml/min/g cotyledon); k₂, first-order efflux rate constant (min^–1); k_s, elimination rate constant (min^–1); V_p, apparent distribution volume of placental compartment (ml/g cotyledon); Q_m, maternal flow rate (ml/min/g cotyledon); Q_f, fetal flow rate (ml/min/g cotyledon); V_m, volume of maternal compartment (23 ml); V_f, intravascular volume of placental tissue (0.06 ml/g cotyledon).

Equations 2 to 5, 2 to 6, and 7 to 9 were simultaneously fittedto the sets of time profiles of maternal and fetal effluents(C_m and C) and the amounts of drug in the perfused tissues (X_p,µg/g cotyledon) in protocols I and Ib, or protocols Iaand II, respectively, by using a nonlinear least-squares program(MLAB; Civilized Software, Bethesda, MD) to obtain transplacentalpharmacokinetic parameters, i.e., K₁ (influx clearance frominterstitial space to placental tissue, ml/min/g cotyledon),k₂ (efflux rate constant from placental tissue to interstitialspace, min^–1), k_s (elimination rate constant from theplacenta, min^–1), and V_p (apparent volume of distributionfrom fetal blood, ml/g cotyledon). X_a represents the amountof drug in the dead volume compartment. V_m and V_f representthe volumes of maternal compartment and fetal intravascularspace (0.06 ml/g cotyledon; Drury et al., 1981

Protocol I, Ia (t $≤$ 62), Ib

Formula (2)

Formula (3)

Formula (4)

Formula (5)
ProtocolIa (62 < t $≤$ 65)

Formula (6)
ProtocolII

Formula (7)

Formula (8)

Formula (9)

Model Analysis for Salicylic Acid (Fig. 3). A pharmacokineticmodel consisting of three placental compartments (i.e., maternalcompartment, placental tissue compartment, and fetal intravascularcompartment) and a dead volume compartment was used to evaluatethe transplacental transfer kinetics of salicylic acid.

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FIG. 3. Pharmacokinetic model of salicylic acid transfer across the placenta observed with a human placental perfusion method. C_in, drug concentration in perfusate (8 µg/ml); C_m, drug concentration in maternal compartment (µg/ml); C, drug concentration in fetal intravascular compartment (µg/ml); X_p, amount of drug in placental compartment (µg/g cotyledon); k_a, first-order influx rate constant (1.02 min^–1); K₁, K₄, influx clearances (ml/min/g cotyledon); k₂, k₃, first-order efflux rate constant (min^–1); k_s, elimination rate constant (min^–1); Q_m, maternal flow rate (ml/min/g cotyledon); Q_f, fetal flow rate (ml/min/g cotyledon); V_m, volume of maternal compartment (23 ml); V_f, intravascular volume in placental tissue (0.06 ml/g cotyledon).

Equations 10 to 13, 10 to 14, and 15 to 17 were simultaneouslyfitted to the sets of time profiles of maternal and fetal effluentsand the amounts of drug in the perfused tissues in protocolsI and Ib, and protocols Ia and II, respectively, by using aleast-squares program (MLAB) to obtain transplacental pharmacokineticparameters, i.e., K₁, k₂, k₃, k₄, and k_s. K₄ and k₃ representthe influx clearance from fetal intravascular space to placentaltissue (ml/min/g cotyledon) and efflux rate constant from placentaltissue to fetal intravascular space (min^–1), respectively.

Protocol I, Ia (t $≤$ 62), Ib

Formula (10)

Formula (11)

Formula (12)

Formula (13)
ProtocolIa (62 < t $≤$ 65)

Formula (14)
ProtocolII

Formula (15)

Formula (16)

Formula (17)

Correction of Kinetic Parameters for Protein Binding in thePerfusate. Protein binding rates of salicylic acid and antipyrinein the perfusate were determined by equilibrium dialysis (Takedomiet al., 1998). The unbound influx clearances from the maternaland fetal sides to the placental tissue (K'₁ and K'₄) were obtainedby dividing the K₁ and K₄ values by the observed free fraction(f_p) of each drug in the respective perfusates. Furthermore,the influx plasma clearances into placental tissue (K''₁ andK''₄) were estimated by multiplying the unbound rate of drugsin the maternal plasma (f_p,m, salicylic acid: 0.568, Hill andAbramson, 1975; antipyrine: 0.884, Ohkawa et al., 2001) andfetal plasma (f_p,f, salicylic acid: 0.457, antipyrine: 0.869).

Results

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Results
Discussion
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Placental Perfusion Technique. Fetal perfusion pressure wasmonitored throughout the experiment and confirmed not to exceed40 mm Hg. Leakage of perfusate from the fetal side was lessthan 3.0 ml/h.

Protocols I and Ia. Antipyrine and salicylic acid appeared rapidlyin the fetal effluent. Their concentrations in the maternaland fetal perfusates reached a steady state within 10 min afterthe start of drug perfusion (Figs. 4 and 5). The TPT_ss valuesof antipyrine and salicylic acid were 7.62% and 4.13%, respectively,showing that the transfer of salicylic acid was 54.2% of thatof antipyrine. In protocol Ia, drug concentrations in the effluentsgradually decreased after the perfusate was changed (Figs. 4and 5).

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FIG. 4. Time courses of antipyrine concentration in effluents during maternal-to-fetal and washout perfusion (protocols I, Ia, and Ib). Closed circles, open circles, and gray diamonds represent the drug concentrations in maternal effluent, fetal effluent, and placental tissue, respectively. Each point represents the mean ± S.D. (n = 3–9).

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FIG. 5. Time courses of salicylic acid concentration in effluents during maternal-to-fetal and washout perfusion (protocols I, Ia, and Ib). Closed circles, open circles, and gray diamonds represent drug concentrations in maternal effluent, fetal effluent, and placental tissue, respectively. Each point represents the mean ± S.D. (n = 3–9).

Protocol II. After the start of drug perfusion, the concentrationof antipyrine in the fetal effluent rapidly reached a steadystate, and the fetal-to-maternal transfer was low (Fig. 6).Fetal-to-maternal transfer of salicylic acid was lower thanthat of antipyrine (Fig. 7).

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FIG. 6. Time courses of antipyrine concentration in effluents during fetal-to-maternal perfusion (protocol II). Closed circles, open circles, and gray diamonds represent drug concentrations in maternal effluent, fetal effluent, and placental tissue, respectively. Each point represents the mean ± S.D. (n = 3).

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FIG. 7. Time courses of salicylic acid concentration in effluents during fetal-to-maternal perfusion (protocol II). Closed circles, open circles, and gray diamonds represent drug concentrations in maternal effluent, fetal effluent, and placental tissue, respectively. Each point represents the mean ± S.D. (n = 3).

Model Analysis. Concentration profiles of antipyrine in thematernal and fetal effluents under protocols I, Ia, Ib, andII were adequately explained by the developed model (Fig. 8).The values of the pharmacokinetic parameters K₁, k₂, and V_pobtained were 0.0791 ml/min/g cotyledon, 0.118 min^–1,and 0.195 ml/g, respectively (Table 1).

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FIG. 8. Model analysis of transplacental transfer of antipyrine. Closed circles, open circles, and gray diamonds represent maternal concentration, fetal concentration, and placental tissue concentration, respectively. The lines represent the model fit (solid line, maternal effluent; dotted line, fetal effluent; dashed line, placental tissue).

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TABLE 1 Transplacental pharmacokinetic parameters of salicylic acid and antipyrine

Each value represents the estimate ± S.D. (68.3% confidence interval).

The concentration profiles of salicylic acid in the maternaland fetal effluents in protocols I, Ia, Ib, and II were alsoadequately explained by the developed model (Fig. 9). The valuesof the pharmacokinetic parameters K₁, k₂, k₃, and K₄ obtainedwere 0.0407 ml/min/g cotyledon, 0.0238 min^–1, 0.176 min^–1,and 0.0813 ml/min/g cotyledon, respectively (Table 1).

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FIG. 9. Model analysis of transplacental transfer of salicylic acid. Closed circles, open circles, and gray diamonds represent maternal concentration, fetal concentration, and placental tissue concentration, respectively. The lines represent the model fit (solid line, maternal effluent; dotted line, fetal effluent; dashed line, placental tissue).

Correction for Protein Binding. The unbound fractions (f_b)ofsalicylic acid and antipyrine in the perfusate were 0.902 and0.932, respectively. The unbound influx clearances of salicylicacid, K'₁ and K'₄, were estimated to be 0.0451 and 0.0901 ml/min/gcotyledon, so that the plasma influx clearances, K''₁ and K''₄,were estimated to be 0.00256 and 0.0412 ml/min/g cotyledon,respectively. Placental tissue-to-plasma concentration ratio,K''₁/k₂, for salicylic acid was estimated to be 1.07 ml/g cotyledon(Table 1).

On the other hand, unbound and plasma influx clearances (K'₁and K''₁) were estimated to be 0.0849 and 0.0751 ml/min/g cotyledon,respectively. Placental tissue-to-plasma concentration ratio,K''₁/k₂, for antipyrine was estimated to be 0.642 ml/g cotyledon(Table 1).

Discussion

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In the present study, we developed a pharmacokinetic model basedon the results of a human placental perfusion study with variousperfusion protocols (protocols II, Ia, and Ib), in additionto the conventional protocol, protocol I (Figs. 8 and 9; Table 1).Each fitting line fell largely within the range of observedvalues ± S.D., and the S.D. value of each parameter didnot greatly exceed the parameter estimate, indicating that themodel fit can be considered adequate.

Distinct models were used to describe the kinetics of antipyrineand salicylic acid in the present study. The model for antipyrineis a variation of that for salicylic acid based on the assumptionthat placental tissue and fetal intravascular space are in rapidequilibrium (Fig. 2). Although we had hoped to apply the modelfor salicylic acid (Fig. 3) directly to antipyrine, the calculatedk₃ and K₄ values were extremely large and failed to converge(data not shown). Therefore, we considered that rapid equilibriumcan be assumed between placental tissue and fetal intravascularspace within the present sampling schedule. Since antipyrineis rapidly distributed into tissues, more frequent samplingmay be required to quantitatively evaluate the kinetics betweenplacental tissue and fetal intravascular space and also to estimatek₃ and K₄ individually. This may also be the case for otherdrugs that are rapidly distributed into tissues.

We assumed a well stirred maternal compartment with a volume(V_m) of 23 ml. Taking into account the maternal flow rate (Q_m)of 15 ml/min, the replacement of fluid in the maternal compartmentis likely to be rapid within the present sampling schedule,and therefore, we assumed the compartment to be well stirred.Although a model involving a concentration gradient (e.g., tubemodel, dispersion model, etc.) might be applicable for eachcompartment, we consider this to be unnecessary for the samereason as above, unless we wish to analyze the kinetics in thesubminute range. On the other hand, the concentration of maternaleffluent reached steady state more slowly than the model describes,suggesting that an additional distribution compartment, whichis adjacent to the maternal compartment, but unconnected tothe fetal compartment, may be involved. However, more complicatedmodels with many parameters failed to converge. Reducing thedead volume (X_a; Figs. 2 and 3), increasing the sampling frequency,and/or using other perfusion protocol(s) may be necessary ifmore complicated models are to be examined.

The calculated transplacental kinetic parameters of salicylicacid and antipyrine obtained with this model are summarizedin Table 1. The unbound influx clearance (K'₁) of salicylicacid was 0.0451 ml/min/g cotyledon, which is about half thatof antipyrine (0.0849 ml/min/g cotyledon). On the other hand,the efflux rate constant of salicylic acid from the placentaltissue to interstitial space (k₂) was 0.0238 min^–1, whichis about one-fifth that of antipyrine. This difference may beexplained by the fact that salicylic acid at physiological pH(7.4) is almost entirely ionized (membrane-impermeable form).The membrane permeability of a drug that does not undergo transporter-mediatedtransport is proportional to the product of the octanol/waterpartition coefficient and (molecular weight)^1/2 (Camenisch etal., 1996). Although this value for salicylic acid at the presentexperimental pH is 0.000562 and far smaller than that of antipyrine(0.136), the observed K'₁ value of salicylic acid was comparableto that of antipyrine, suggesting that the K'₁ value of salicylicacid is larger than would be predicted from its physicochemicalproperties. Therefore, transplacental transfer of salicylicacid may be mediated by a specific system, at least in part.Indeed, we have shown that BeWo cells, a human placental choriocarcinomacell line, take up salicylic acid together with protons viaa specific transport system (Emoto et al., 2002). A known proton-dependenttransporter, monocarboxylate transporter 4, is highly expressedon the maternal side of human placental trophoblasts (Settleet al., 2004). Thus, proton-dependent transporter(s) such asmonocarboxylate transporters may contribute to the transplacentaltransport of salicylic acid.

In the present model analysis, the value of the parameter, k_s,which represents the elimination of drug from the placenta,was derived from the mean recovery of antipyrine (82.6%). Antipyrinehas been used as a typical passive diffusion marker in humanplacental perfusion studies. However, we also retrospectivelycalculated the recovery from the antipyrine concentrations inthe influx perfusate and effluents in other studies, and foundthat it was generally less than 100%, i.e., 80% in the caseof Schenker et al. (1992), 70% according to Lampela et al. (1999),and 75% in the study by Nanovskaya et al. (2002). A likely explanationis metabolism of antipyrine in the placenta. Although thereis no report concerning metabolism of antipyrine in the placenta,antipyrine is metabolized by a variety of cytochrome P450 isoformssuch as CYP1A2, 2B6, 2C8, 2C9, 2C18, and 3A4 (Engel et al.,1996; Carcillo et al., 2003), and the placenta is known to expressCYP3A4 protein and mRNAs of CYP1A2 and CYP2C family members(Hakkola et al., 1996; Pasanen, 1999). Thus, the rate constant,k_s, may include a contribution from metabolism of antipyrinein the placenta. On the other hand, the k_s value for salicylicacid was quite small (1.81 x 10^–4 min^–1), suggestingthat it may not be metabolized in the placenta.

We used four protocols (protocols I, II, Ia, and Ib) of humanplacental perfusion. Whereas most human placental perfusionstudies have been done at steady state, a non-steady-state modelwas applied to the time-profiles of the drug concentrationsin the effluent. Our model with frequent sampling after thestart of drug perfusion could provide kinetic parameters suchas K₁. Protocol II is considered to have been helpful to preciselycalculate the parameters k₃ and K₄, because in the absence ofthe results of protocol II, these parameters could not be accuratelyestimated (data not shown). In other words, observation of transferkinetics of a drug from maternal perfusate to fetal effluentis not sufficient to allow evaluation of the kinetics of drugtransfer among interstitial space, placental tissue and fetalintravascular space. Protocol Ia was helpful to evaluate theefflux of the drug from placental tissue to the effluents, i.e.,k₂ and k₃, more accurately. Although we did not evaluate theacceptability of the precision by using any index, the relativeS.D. value of k₂, especially for salicylic acid, was largerthan those of other parameters. This may reflect the existenceof a maternal dead volume compartment (X_a; Figs. 2 and 3), whichmay weaken the concentration clamp of the maternal perfusate.Protocol Ib was also helpful to determine the initial drug uptakerate from maternal perfusate to placental tissue. Although thedrug amount in the placental tissue can theoretically be obtainedat steady state from a mass-balance equation, if the drug isnot eliminated in the placenta, the tissue sampling indicatesthat antipyrine may be eliminated in the placenta. In protocolII, the model underestimated the concentration-time profilesof the fetal effluents (Figs. 8 and 9). This seems to be consistentwith the observation that the recovery rates of drugs ([C_m ·Q_m + C · Q_f]/C_in · Q_in) in protocol II were higherthan those in protocol I. Although the reason for this differenceremains to be elucidated, a possible explanation is that somefactor(s), such as a heterogeneous enzyme distribution in theplacental tissue, leads to differences in the metabolic capacityfor the drug between protocols. In any case, simultaneous fittingof the model to the sets of concentration profiles and tissueconcentrations enabled us to determine the transplacental parameterswith sufficient accuracy.

Our model allowed us to evaluate the elemental processes oftransplacental transfer of salicylic acid. This in turn makesit possible to predict the influx profile of the drug into fetalumbilical veins by using the plasma concentration-time profileof the drug in gravidae. The present model analysis may thereforeprovide clinically significant information about fetal exposureto drugs given to the mother during full-term gestation, andmay be applicable to the prediction of possible fetal toxicityof diclofenac, digoxin, paroxetine, and so on. It may also bepossible to evaluate the physiological contributions of certaintransporter(s) to the transplacental transfer of drugs by thepresent technique, if a specific inhibitor of the transporteris perfused simultaneously with the substrate. Moreover, ifthe placental transfer is altered by some factor (e.g., pathology,genotype, concomitant drug administration, etc.), the presentmodel-based analysis may be useful to reveal what process wasaffected. We may also simulate the effects of change in an individualprocess (e.g., change in drug transporter function) on the overalltransfer function of the placenta.

In conclusion, the time profiles of the concentration of salicylicacid in the effluents under various protocols of placental perfusioncan be adequately explained by our newly developed pharmacokineticmodel. The model analysis provided the transplacental transferkinetics of salicylic acid and enabled us to estimate the influxprofile of the drug into the fetal umbilical vein from the plasma-concentrationprofile of the drug in the gravidae.

Footnotes

This study was supported in part by grants from Japan HumanSciences Foundation and Japan Society for the Promotion of Science(JSPS).

Article, publication date, and citation information can be foundat http://dmd.aspetjournals.org.

doi:10.1124/dmd.106.013029.

ABBREVIATIONS: HPLC, high-performance liquid chromatography;TPT_ss, ratio of the rate of amount transferred across the placentato that infused in the steady state.

Address correspondence to: Yasufumi Sawada, Department of Drug Informatics, Graduate School of Pharmaceutical Sciences, The University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan. E-mail: sawada{at}mol.f.u-tokyo.ac.jp

References

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