Background
Malaria is one of the deadliest infectious diseases in the world, causing nearly a million deaths among more than three billion people who were at risk in 2006 [
1]. Unfortunately, given the high burden of the disease, the number of available anti-malarial drugs is relatively small. On top of that, the emergence of resistance to the most affordable anti-malarial drugs has seriously undermined the global effort to control malaria. As the result of chloroquine and sulphadoxine-pyrimethamine resistance, millions of lives that could otherwise be saved were sacrificed over the past 30 years [
2]. Artemisinin-based combination therapy (ACT) is now being widely used as the first-line treatment for
Plasmodium falciparum malaria throughout the world.
Artemisinin (ARN) and its derivatives, dihydroartemisinin (DHA), artesunate (AS), artemether and arteether are fast acting anti-malarial drugs producing the most rapid reduction in parasitaemia [
3]. These agents also have gametocytocidal activity, which contributes to the reduction in the disease transmission [
4,
5]. Among the available derivatives, AS has the most appealing physicochemical and pharmacological properties. It is more water soluble, thermally and chemically more stable, and rapidly converted
in vivo to its active metabolite DHA, which is responsible for most of the anti-malarial activity [
6,
7].
Pyronaridine (PYR) is a Mannich-base derivative anti-malarial that has been shown to be efficacious against erythrocytic stages of
P. falciparum using
in vitro models [
8‐
10]. Clinical studies have also indicated that PYR is safe and efficacious against
P. falciparum even in area with chloroquine-resistant strains [
11‐
13]. Pyronaridine tetraphosphate plus artesunate (PA) is under development as a 3:1 fixed ratio combination for the treatment against
P. falciparum and
P. vivax malaria.
Population pharmacokinetics of AS and/or DHA following the administration of AS have been previously described in malaria patients. Karunajeewa and colleagues investigated the disposition of AS and DHA in 47 children from Papua New Guinea with uncomplicated malaria after the administration of AS suppositories [
14]. The population pharmacokinetics of DHA were also assessed in 164 patients with moderately severe falciparum malaria following intra-rectal dosing of AS, in 24 pregnant women and in 70 African children with acute uncomplicated falciparum malaria after the administration of oral AS [
15‐
17]. However, parent AS data were not modelled in these two studies, mainly because there were too few data points available for AS.
To date, no population pharmacokinetics analysis of AS and DHA has been published in healthy subjects receiving oral AS dosing. Such analysis will provide a means of comparing the pharmacokinetics of AS and DHA in malaria patients and healthy subjects and, therefore, expand the understanding in the effect of the disease state on the pharmacokinetics of AS and DHA. The aims of this analysis are to develop a population pharmacokinetic model of AS and DHA in healthy subjects following oral administration of PA combination or AS alone and to identify covariates that are important determinants of the variability seen in pharmacokinetic parameters of AS and DHA.
Methods
Subjects and study designs
Data used in performing this analysis were pooled from a four-part Phase I clinical trial (Protocol number SP-C-001-03). The trial was conducted at the Clinical Trial Center of Seoul National University, Seoul, South Korea, in accordance with the Guidelines of Good Clinical Practice and Declaration of Helsinki. Ethical approval was obtained from Institutional Review Board of Seoul National University. Written informed consent was obtained from each subject prior to the studies. All subjects were healthy Korean men and women evaluated by a physician at screening (Day -21 to -2) based on physical examination, vital signs, electrocardiogram, medical history and laboratory evaluations. All study drugs and placebos were provided by Shin Poong Pharmaceuticals (Seoul, Korea) and were identical in appearance to maintain blinding.
The first part was designed as a single oral ascending dose, randomized, double-blind, placebo-controlled, staggered and parallel group study to evaluate the pharmacokinetics, safety and tolerability of PA following single oral administration of PA at following doses: 6+2 mg/kg, 9+3 mg/kg, 12+4 mg/kg or 15+5 mg/kg. Nine subjects were recruited for each dose level, and randomized to receiving either PA treatment or placebo in 7:2 ratio.
The second part was conducted to evaluate the potential of drug interaction between PYR and AS when used as a combination in 3:1 ratio. It was a two-cohort parallel, two-period randomized, blinded, crossover study of a single oral dose of PA 12+4 mg/kg versus each of the individual drug at the same dose plus placebo of the other drug. 20 subjects were enrolled into this study, and randomly assigned into either cohort 1 or cohort 2 in equal numbers. In cohort 1, five subjects received PYR alone in period 1 followed by PA combination in period 2, while another five received the treatments in reverse order. In cohort 2, five subjects received AS alone in period 1 followed by PA combination in period 2, while another five received the treatments in reverse order. There was a 21-day washout period between the two periods.
The third study was a two-period, randomized and cross-over study to investigate the effect of food on the pharmacokinetics of PA. 20 subjects were enrolled into the study and randomly allocated to each of the fasted or the fed arm in equal numbers. After an overnight fast of at least 10 hours, the subjects in the fasted arm received PA 12+4 mg/kg with 240 mL of water and remained fasted for at least 4 hours post-dose while the subjects in the fed arm ingested a high-fat and high-caloric test meal 30 minutes prior to the treatment. After a washout period of 21 days, the subjects returned for the crossover treatment. Water was permitted as desired, except for one hour before and after drug administration, and a standard meal was scheduled at the same time in each period of the study for each subject.
The purpose of the last part of trial was to evaluate the pharmacokinetics, safety and tolerability of PA following multiple oral dosing of PA at following doses: 6+2 mg/kg, 9+3 mg/kg, 12+4 mg/kg or 15+5 mg/kg once daily for three consecutive days. The study design was otherwise similar to the design of the first study. Eight subjects were recruited for each dose level, and randomized to receiving either PA treatment or placebo in 6:2 ratio.
Sample collection and storage
For the first three studies, venous blood samples for the determination of AS and DHA pharmacokinetics were collected prior to dosing and at 0.33, 0.67, 1.33, 1.67, 2, 2.5, 3, 4, 5, 8 and 12 hours post-dose. For the multiple-dosing study, the samples were taken prior to the dosing of each dose and at 0.33, 0.67, 1, 1.33, 1.67, 2, 2.5, 3, 4, 5, 8 and 12 hours after the third dose. Blood samples were collected into pre-chilled sampling tubes containing potassium oxalate/sodium fluoride (BD Vacutainer systems, Franklin Lakes, NJ) and placed on wet ice before centrifugation within five minutes of collection. Immediately after centrifugation, plasma was removed and transferred into two approximately equal volume aliquots in screw cap Nalgene cryovials and then frozen immediately at or below -80°C until analysis.
Analytical method
Plasma concentration of AS and DHA were determined using a validated liquid chromatography-mass spectrometric method described by Naik
et al[
18]. All samples were assayed in the same laboratory. The plasma samples spiked with internal standard ARN was cleaned up using solid phase extraction method. Analysis was performed with a Shimadzu Model 2010 liquid chromatograph-mass spectrometer (Shimadzu, Columbia, MD) in single ion monitoring positive mode using atmospheric pressure chemical ionization as an interface. The lower limit of quantification for AS and DHA using 0.5 mL of plasma was 1 ng/mL. The coefficient of variation for intra-day and inter-day precision ranged from 7% to 14% and 9% to 14% for AS, and 11% to 14.9% and 11% to 15% for DHA, respectively.
Population pharmacokinetic analysis
Nonlinear mixed-effect model building was conducted using NONMEM software version VI, level 2.0 (ICON Development Solutions, Ellicott City, MD) [
19], as implemented on a Windows XP operating system (Microsoft Corporation, WA, Seattle) with G95 Fortran compiler (Free Software Foundation, Boston, MA). All models were fitted using the first-order conditional estimation method. NONMEM output was processed using PDx-Pop 3.10 (ICON Development Solutions, Ellicott City, MD) and Xpose version 4.0 (Uppsala University, Uppsala, Sweden) [
20]. Graphical plots were produced using S-PLUS version 8.0 (Insightful Inc, Seattle, WA) and R 2.8.1 (Free Software Foundation, Boston, MA).
Measurements below the lower limit of quantification of the assay were excluded from the dataset. Since the molecular weights of AS and DHA are quite different (384.4 for AS and 284.9 for DHA), the concentrations were converted to the equivalent values in nmols/L. AS dose was also converted to the equivalent values in nmols. The concentrations were then natural log-transformed before the analysis.
Model selection was guided by the plausibility of the estimates, minimum objective function value (OFV), equal to minus twice the log-likelihood function, Akaike Information Criterion (AIC), equal to OFV plus two times the number of parameters, condition number, defined as the ratio of the largest Eigen value to the smallest Eigen value, visual inspection of diagnostic plots and the precision of parameter estimates.
In the initial stage of model building, one- and two-compartment pharmacokinetic models with first order absorption and first order elimination were fitted to the AS data to determine the best structural model for AS. Once the best pharmacokinetic model for AS was determined, DHA data was modelled as a metabolite compartment connected to the central compartment of AS. It was assumed that conversion to DHA was the only significant route of elimination for AS and that the conversion was irreversible [
21]. One- and two-compartment models with first-order disposition were tested for DHA to develop the best metabolite structural model. For the two-compartment model, it was assumed that DHA was eliminated only from the central compartment. After the best structural model was determined, all parameters were estimated simultaneously using ADVAN 6 in NONMEM.
Inter-individual variability (IIV) of the pharmacokinetic parameters was modelled assuming a log-normal distribution, as follows:
where Pi is the estimated parameter value for individual i, Ppop represents the typical population estimate for the parameter and ηi is the deviation of Pi from Ppop. The η random effects were assumed to be independent and symmetrically distributed with zero mean and variance ε2. A diagonal covariance matrix was modelled, as the data did not support the implementation of a full variance-covariance matrix. The magnitude of IIV was expressed as coefficient of variation (%CV), which was approximated by the square root of the variance estimate.
Residual variability (RV) was modeled using an additive model as shown below:
where Cij and Cpred, ij represent the jth observed and model predicted AS or DHA concentrations, respectively, for individual i and εij denotes the additive residual random error for individual i and observation j. The ε random effects were assumed to be independent and symmetrically distributed with zero mean and variance σ2.
After the optimum model for AS and DHA was determined, covariate analysis was carried out to assess additional variables as possible determinants of the variability seen in the pharmacokinetic estimates. Covariates examined include total body weight, age, gender, type of dosing (single- or multiple-dosing), treatment (co-administration of PYR) and food intake (fasted or fed). A summary of the covariates evaluated is shown in Table
1. Potential covariates were initially identified using generalized additive modelling (GAM) as implemented in the Xpose software. The potential covariates were then tested using stepwise forward addition followed by stepwise backward elimination procedure [
22]. The influences of the covariates were tested by adding a covariate to the model at a time in the forward addition step, and then by removing a covariate from the model at a time in the backward elimination step. The changes in OFV between the 'full' and the 'reduced' models were then calculated. The difference in OFV between two nested models was approximated by a χ
2 distribution. An OFV change of 3.84 (corresponding to a significance level of 5% at one degree of freedom) was used as the cut-off to include a covariate in stepwise addition. When no more covariates could be included, the stepwise backward elimination was carried out. For a covariate to remain in the model, a change in OFV of at least 10.83 (corresponding to a significance level of 0.1% at one degree of freedom) was needed.
Table 1
A summary of the study data, subject demographics and covariates included in the analysis.
No. of subjects | 28 | 19 | 20 | 24 | 91 |
No. of concentration-time profiles | 28 | 28 | 38 | 24 | 118 |
No. of observations | | | | | |
AS | 206 | 207 | 324 | 179 | 916 |
DHA | 316 | 314 | 449 | 273 | 1352 |
AS dose (mg/kg) | 2, 3, 4 or 5 | 4 | 4 | 2, 3, 4 or 5 | 2, 3, 4 or 5 |
Sampling schedule | Predose, 0.33, 0.67, 1, 1.33, 1.67, 2, 2.5, 3, 4, 5, 8 and 12 h postdose | Predose, 0.33, 0.67, 1, 1.33, 1.67, 2, 2.5, 3, 4, 5, 8 and 12 h postdose | Predose, 0.33, 0.67, 1, 1.33, 1.67, 2, 2.5, 3, 4, 5, 8 and 12 h postdose | Immediately prior to each dose and 0.33, 0.67, 1, 1.33, 1.67, 2, 2.5, 3, 4, 5, 8 and 12 h after the third dose | NA |
Age (years) | 24 (19-40) | 23 (20-32) | 21.5 (19-27) | 23 (19-29) | 23 (19-40) |
Weight (kg) | 62.5 (50.4-70) | 60.9 (50.1-67.1) | 59.9 (50.8-68.5) | 62.2 (51.2-68.8) | 61.5 (50.1-70) |
Sex (number) | | | | | |
Female | 9 | 10 | 10 | 9 | 38 |
Male | 19 | 9 | 10 | 15 | 53 |
Type of dosing | Single | Single | Single | Multiple (once daily for 3 days) | NA |
Food intake (number of profiles) | | | | | |
Fasted | 28 | 28 | 19 | 24 | 99 |
Fed | 0 | 0 | 19 | 0 | 19 |
The relationship between continuous covariates and pharmacokinetic parameters were evaluated using both linear and power functions, with the covariates centered or scaled at their median values:
where θ
1 represents the parameter estimate P of an individual with a body weight of 61.5 kg and θ
2 is a factor describing the correlation between body weight and the parameter. The influences of binary covariates on the parameter were modelled using a proportional relationship, as follow:
where θ3 represents the parameter value in subjects receiving the test drug without food, and θ4 is the fractional change in the parameter in subjects receiving the test drug with food. FOOD variable was coded as 0 for the fasted subjects and 1 for the subjects who received test drug with food.
Model evaluation
The non-parametric bootstrap procedure was employed to evaluate the precision of the parameter estimates and the robustness of the final model. 500 bootstrap datasets were generated by repeated random sampling with replacement from the NONMEM input data file, and the final NONMEM model was fitted to the bootstrap datasets. Bootstrap parameter estimates, standard errors and 95% confidence intervals were obtained and compared with the parameter estimates from the original dataset.
Visual predictive check was also performed to evaluate the predictive ability of the model. 500 virtual observations at each sampling time point were simulated using the final model and its parameter estimates. The observed data were then plotted with the 5th, 50th and 95th percentiles of the simulated data that was above the limit of quatification. The percent of observations outside the 90% prediction interval was also calculated. The condition number of the final model was also calculated as a measure of the stability of the model.
Discussion
In the current analysis, a novel parent-metabolite model to describe the population pharmacokinetics of AS and DHA in healthy subjects was developed. This is the first population pharmacokinetic analysis of AS and DHA conducted using data derived from a large number of healthy subjects following oral administration of AS. The model developed was stable and was able to predict AS and DHA data arising from single- and multiple-dosing of oral AS equally well.
AS was rapidly absorbed into the systemic circulation, with an absorption half-life of 10.8 minutes estimated in this analysis. The conversion of AS to DHA was very rapid and the concentration of DHA was measurable as early as 20 minutes post-dose for all subjects. The sensitivity of the assay used in this study enabled the measurement of AS concentrations up to eight hours post-dose and the measurement of DHA concentrations up to 12 hours post-dose, in 65% and 95% out of the total 1416 available samples, respectively. Therefore, we were able to characterize the distribution of lipophilic DHA to the peripheral tissue. The pharmacokinetic parameter estimates obtained using a non-linear mixed-effects modelling approach employed in this analysis are comparable with those obtained using non-compartmental analysis (unpublished data).
The pharmacokinetics of AS and DHA following orally administered AS in healthy subjects have been previously reported in different settings [
23‐
26]. However, AS pharmacokinetics was not described in the reports by Benakis
et al[
23] and Na-Bangchang
et a l [
26]. Navaratnam
et al[
24] compared the pharmacokinetics of AS and DHA after administration of oral and rectal AS in 12 healthy male Malaysian volunteers using non-compartmental approach. Following a single oral dose of 200 mg AS, the mean area under the plasma concentration-time curve (AUC) to time infinity for AS was reported to be 119 ng.h/mL, corresponding to a CL/F of 1680 L/h. A lower CL/F for AS (1190 L/h) was reported in the current analysis using data from a much larger sample size. The bioanalytical method used to measure AS plasma concentrations was also more sensitive (limit of quantification = 1 ng/mL) in current analysis. Teja-Isavadharm and colleagues [
25] studied the single-dose pharmacokinetics of AS following the administration of 100 mg of oral AS in six healthy subjects and six patients with uncomplicated falciparum malaria. In their study, the range of apparent clearance and apparent volume of distribution in healthy subjects were 4.69-29 L/h/kg and 4.2-49.6 L/kg for AS, 1.66-3.26 L/h/kg and 1.99-4.45 L/kg for DHA, respectively. The weight normalized apparent clearance and apparent volume of distribution obtained in this analysis were 19.3 L/h/kg and 19.7 L/kg for AS, 1.52 L/h/kg and 1.88 L/kg for DHA, respectively. The estimates obtained in this present analysis are within the similar magnitude compared to their findings.
Several other studies have described the pharmacokinetics of DHA following the administration of oral AS in malarial patients [
27‐
29]. Newton
et al studied the disposition of DHA in 19 adult patients with acute uncomplicated falciparum malaria who were treated with 2 mg/kg of oral AS [
29]. DHA data was modelled using an open one-compartmental model with first order absorption and elimination assuming complete conversion of AS to DHA. The reported CL/F and V/F values were 73.1 L/h and 70.5 L, respectively. In another study, the pharmacokinetic characteristics of DHA were described in 26 malarial patients who received 100 mg of oral AS, using non-compartmental analysis [
28]. The reported AUC and t
1/2 of DHA were 4.53 μmols.h/L and 0.66 h, respectively. These values correspond to a CL/F of 51.7 L/h and a V/F of 48.9 L. Similarly, Bethell
et al reported the AUC and t
1/2 of DHA of 1286 ng.h/mL and 1 h, respectively, in 10 children with moderately severe falciparum malaria who received 3 mg/kg of oral AS [
27]. These values correspond to a CL/F of 45.7 L/h and a V/F of 65.9 L. All these values for CL/F and V/F of DHA were lower than the value reported in this analysis. These differences could be resulted from the use of different assays, the effect of disease state (malaria), differences in the dose formulations, and/or the age-related difference in DHA metabolism capacity.
Population pharmacokinetics of AS and/or DHA in malaria patients have been described in four other papers [
14‐
17]. Karunajeewa
et al[
14] proposed a three-compartment model (a rectal absorption compartment, a central compartment for AS and a central compartment for DHA) to describe the population pharmacokinetics of AS and DHA simultaneously in paediatric patients following administration of AS suppositories. Simpson
et al[
16] modelled only the DHA data pooled from five Phase II and III studies conducted in adult and paediatric malaria patients. Both the weight-normalized CL/F and V/F for AS obtained in our analysis are much larger than the ones reported by Karunajeewa
et al (5.9 L/h/kg and 2.1 L/kg, respectively) [
14]. The larger CL/F and V/F for AS seen in our study might be attributed to the fact that the AS bioavailability is reduced when oral AS is given compared to rectal AS [
24]. On the other hand, the weight-normalized CL/F and V/F for DHA obtained in this study are smaller than those reported by the two studies. Karunajeewa
et al reported values of 2.2 L/h/kg and 2.1 L/kg for the CL/F and V/F of DHA [
14]. The typical CL/F values of DHA reported by Simpson
et al were 3.17 L/h/kg for a male and 2.03 L/h/kg for a female. For an adult weighted 70 kg, the typical value for V/F of DHA was 6.34 L/kg [
16]. This finding is also consistent with the observations that the AUC for DHA following oral administration of AS was higher than that following rectal AS [
24,
30], suggesting that the bioavailability of DHA was increased when oral AS was given.
McGready
et al[
15] characterized the population pharmacokinetics of DHA in pregnant women with acute uncomplicated falciparum malaria following a three-day dosing of oral AS (4 mg/kg/day) and atovaquone plus proguanil. However, the pharmacokinetics of AS was not evaluated because AS was detectable only in about 6.5% of the total available samples. The pharmacokinetic parameter estimates for DHA were therefore derived using AS dose in DHA equivalents. The CL/F of DHA was reported to be 1.77 L/h/kg, which is similar in our analysis. However, the estimate for DHA apparent volume of distribution in healthy Korean subjects obtained in this analysis is about 60% lower compared to the pregnant Karen patients in their study (4.63 L/kg). The larger volume of distribution seen in their study might be attributed to the physiological changes during pregnancy and the effect of the disease state.
Stepniewska
et al conducted a population pharmacokinetic study of AS in African children with acute malaria from six months to five years old [
17]. The subjects received either the fixed dose combination of AS and amodiaquine or the separate tablets of both drugs. The DHA data was modelled using nonlinear mixed-effects approach. The weight normalized CL/F of DHA reported in their study was 0.636 L/h/kg, which was almost 60% lower than the value analysis in healthy adults. The discrepancy could be related to the developmental changes of metabolizing enzymes that take place in the young children. It has been demonstrated that the glucuronidation of DHA was catalyzed by UDP-glucuronosyltransferases (UGTs), in particular UGT1A9 and UGT2B7 [
21]. The capacity of these metabolizing enzymes in young children could be much less than the full capacity in adults [
31] and therefore resulted in lower CL/F of DHA. In a review on developmental patterns of UGT system, de Wildt
et al suggested that the use of per-kg model for clearance is adequate to address developmental changes in young children and may lead the underestimation of clearance by up to 200% in chilren under 3.4 kg of body weight [
31]. The reported weight-normalized V/F of DHA by Stepniewska
et al was 2.285 L/kg [
17], which was quite similar to the value obtained in this analysis.
In the present analysis, food intake was found to significantly delay the absorption of AS. When AS dose was administered after the intake of high-fat and high-caloric meal, the population absorption half-life of AS increased from 10.8 minutes to 67.5 minutes. However, the extent of absorption was not altered significantly. Body weight affected CLM/F significantly and therefore was included as a covariate in the final model. The average CLM/F for a healthy subject with 61.5 kg of body weight was estimated to be 93.8 L/h. A unit deviation in body weight would result in 1.9 unit deviation in the CLM/F from the population estimate. None of the other covariates tested was significant determinants of the variability seen. Co-administration of PYR did not affect any of the pharmacokinetic parameters of AS and DHA.
Remarkable time-dependent pharmacokinetics of ARN has been observed in both healthy subjects and in malaria patients after single or repeated oral and rectal administration of ARN dose [
32‐
35]. Auto-induction of CYP2B6 and CYP2C19 was proposed to be the main mechanism causing the decline of plasma ARN concentrations [
36‐
38]. A semi-physiological pharmacokinetic model taking into account the autoinduction phenomenon has been developed for ARN in healthy subjects [
39]. Conflicting observations have been reported concerning the autoinduction phenomenon after the administration of AS dose. In their unconvincing report, Khanh
et al[
40] observed a decline in DHA concentrations in 6 malaria patients following repeated AS dosing. However, the decline in either AS or DHA concentration was not observed in two other studies [
41,
42]. In this analysis, the type of dosing was tested in the covariate analysis to investigate any differences in the pharmacokinetics of AS and DHA following the administration of single- and multiple-dose of AS. None of the AS and DHA pharmacokinetic parameters was affected by the type of AS dosing received at a significance level of 0.05. Visual predictive check plots in Figure
4 shows similar distributions for AS and DHA observations following single- or multiple-dose of AS, indicating no sign of decline in AS and DHA concentrations after three repeated daily AS dosing. The model described the AS and DHA observations equally well regardless the type of dosing received by the healthy subjects. In addition, the mean AS/DHA AUC
0-8 ratios were similar after single and multiple doses (0.10 and 0.11, respectively). This provides evidence that there is little or no induction of the metabolic enzymes involved in the metabolism of AS following once daily dosing over three days.
Authors' contributions
BT conducted the pharmacokinetic modelling and drafted the manuscript. HN conducted the bioanalysis of the artesunate plasma samples. IJJ and KSY carried out the clinical aspects of the study including the acquisition of data. BT, HN, LF and LK participated critically in discussions throughout the modelling process and interpretation of pharmacokinetic data. IJJ, CSS, JCC and LF contributed substantially to the concept and design of the clinical trial and were part of the protocol development team. All authors critically reviewed the manuscript and approved the final version of the manuscript for submission.