![[Feedback]](/icons/banner/feedbackACT.gif){kind=icon}
![[For Subscribers]](/icons/banner/subscriberACT.gif){kind=icon}
![[Archive]](/icons/banner/archiveACT.gif){kind=icon}
![[Search]](/icons/banner/searchACT.gif){kind=icon}
![[Contents]](/icons/banner/tocACT.gif){kind=icon}
|
|
|
|
|
||
Vol. 285, Issue 1, 71-82, April 1998
-Acetylmethadol:
Pharmacodynamics and Pharmacokinetics in Humans1
Behavioral Pharmacology Research Unit, Department of Psychiatry and Behavioral Sciences, Johns Hopkins University School of Medicine, Baltimore, Maryland
 |
Abstract |
|---|
Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
Levo-
-acetylmethadol (LAAM) is a long-acting opioid agonist approved
for use as a maintenance treatment for opioid dependence. Previous
clinical studies report that the onset of the effects of LAAM is slower
after parenteral administration than oral administration; however,
preclinical studies suggest otherwise. This study examined the
pharmacodynamic and pharmacokinetic profile of LAAM when given orally
and intravenously to humans. Opioid-experienced volunteers (n = 6), who were not physically dependent on
opioids, received LAAM (20 and 40 mg/70 kg i.v. and p.o.) and placebo
under double-blind, double-dummy conditions during five weekly
experimental sessions. Behavioral, physiological, subjective and
pharmacokinetic measures were collected before and for 96 hr after drug
administration. Intravenous LAAM produced significant subjective and
physiological effects that appeared within 5 min, whereas the effects
of oral LAAM appeared more slowly within 1 to 2 hr after drug
administration. Pharmacokinetic data indicate that the immediate
effects of intravenous LAAM are largely attributable to the parent drug
rather than the active metabolites, nor-LAAM and dinor-LAAM. LAAM
produced prototypic opioid agonist effects (i.e.,
miosis, subjective ratings of high, nodding) that were of equal
magnitude across routes, dose-related and of long duration (up to 60 hr). These data are in contrast to previous clinical reports and
indicate that LAAM produces effects of immediate onset when
administered parenterally, which suggests that intravenous LAAM
possesses greater abuse potential than previously believed.
| |
Introduction |
|---|
|
Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
Levo--acetylmethadol
is a synthetic opioid that was approved for use as a treatment for
opioid dependence by the Food and Drug Administration in 1993. A
congener of methadone, LAAM produces opioid effects typical of
mu agonists, including analgesia, euphoria, miosis and
respiratory depression (Fraser and Isbell, 1952
; David and Semler,
1952). Compared with other mu opioid agonists, LAAM has an
exceptionally long duration of action and can produce effects lasting
up to 72 hr after a single acute dose (Fraser and Isbell, 1952). This
long duration of action has enabled clinicians to administer LAAM to
opioid-dependent patients with less-than-daily dosing schedules and to
achieve adequate suppression of withdrawal symptoms when administering
LAAM as infrequently as three times weekly (Ling et al.,
1975; 1976; Senay et al., 1977; Freedman and Czertko, 1981).
The persistent action of LAAM has been attributed primarily to its
sequential N-demethylation to two primary active metabolites, nor-LAAM
and dinor-LAAM (McMahon et al., 1965; Billings et
al., 1973, 1974; Henderson et al., 1977a). Although
N-demethylation by cytochrome P450 3A4 apparently serves as the primary
metabolic path (Moody et al., in press), LAAM may also be
deacetylated to form methadol and normethadol (see Kaiko and Inturrisi,
1975; Chiang et al., 1995). norLAAM and dinorLAAM are
present in plasma for up to 72 to 96 hr after acute or chronic dosing
with LAAM in animals (Henderson et al., 1977a) and humans
(Kaiko and Inturrisi, 1975; Henderson et al., 1977b),
whereas the parent drug is no longer detected. Although LAAM has a
half-life estimated to range from 4.6 to 7 hr, the half-lives of
nor-LAAM and dinor-LAAM are estimated to range up to 48 hr and 4 or
more days, respectively (Henderson et al., 1977c; Kaiko and
Inturrisi, 1975; Chiang et al., 1995). Reports suggest that
nor-LAAM is 5 to 10 times more potent than LAAM and dinor-LAAM in a
variety of assays (Nickander et al., 1974; Billings et
al., 1973; Perez-Reyes, 1985). Thus, the potency and long duration
of action of LAAM has been attributed, in large part, to these
long-acting active metabolites.
The earliest clinical studies of LAAM reported the unusual finding that
the effects of LAAM administered parenterally were delayed in onset in
comparison with those of orally administered LAAM. Oral administration
of LAAM at doses of 30 to 40 mg produced measurable effects within 1 hr, whereas detectable opioid effects were not observed until up to 4 to 6 hr after intravenous or subcutaneous LAAM at 10 to 30 mg (Fraser
and Isbell, 1952; Fraser et al., 1954). This finding is
antithetical to the predicted relationship between the rate of drug
delivery and the onset of pharmacodynamic effects; typically the onset
of drug action is fastest after administration by a parenteral route
(e.g., Benet et al., 1991). To explain this atypical finding, it was hypothesized that the parent drug LAAM was
inactive and that the parenteral delivery of the drug slowed the rate
of metabolism and formation of the active metabolites. Statements
characterizing LAAM as an inert prodrug and descriptions of its delayed
parenteral effects have been included in widely used pharmacology texts
(e.g., see Jaffe and Martin, 1991; Jaffe, 1992). These data
also contributed to regulatory decisions that restricted take-home
doses of LAAM because of the presumed risk of toxic interactions
between supplemental illicit opiates used after oral LAAM.
In contrast to the widely cited report by Fraser and Isbell in 1952, another clinical study on LAAM published in the same year went
relatively unnoticed (Keats and Beecher, 1952). In that study the
analgesic efficacy of LAAM was evaluated in postsurgical patients who
received acute doses of LAAM subcutaneously. LAAM (5-20 mg) was
modestly effective at producing analgesia. Importantly, there was no
significant delay in the analgesic response in contrast to the delayed
"euphoric" response observed by Fraser and Isbell (1952).
Conflicting findings regarding the differential latency of the onset of
parenteral versus oral LAAM also have been reported in
laboratory animals. Studies in monkeys and dogs have reported that the
time to onset of effects for intravenous and intramuscular LAAM is
similar to that of oral LAAM (i.e., 30 min to 1 hr post-drug administration) on various dependent measures including analgesia, sedation and electroencephalographic effects (Henderson, 1976a; Killam,
1976; Lukas et al., 1980; see also Archer, 1976). In another study, the relative analgesic potencies of LAAM, nor-LAAM and dinor-LAAM were compared with the mouse writhing assay (Smits, 1974).
The analgesic effects of LAAM were apparent within 1 hr after
subcutaneous administration, although the response to LAAM was somewhat
slower than that of nor-LAAM or dinor-LAAM. Similarly, LAAM was
pharmacologically active, although less potent, than nor-LAAM and
dinor-LAAM in the guinea pig ileum twitch assay (Nickander et
al., 1974). In this case, use of an isolated tissue preparation precluded appreciable biotransformation of LAAM to its active metabolites. These studies suggest that the parent drug LAAM is an
active drug and that LAAM can produce effects shortly after parenteral
administration which are not caused by its metabolic transformation to
nor-LAAM and dinor-LAAM.
In summary, there are conflicting findings from studies evaluating the relative time to onset of the effects of parenteral and oral LAAM. The early clinical studies cited herein were published largely as descriptive case reports and were conducted before the development of rigorously controlled, double-blind laboratory procedures and the use of standardized subjective and objective rating measures. To date, there have been no contemporary studies assessing the pharmacodynamic and pharmacokinetic profiles of oral and parenteral LAAM in humans. Because of the discrepancies between prior reports regarding the onset of parenteral LAAM effects, the present laboratory study was undertaken to reevaluate the effects of LAAM in humans. This study was designed to characterize and compare the acute pharmacodynamic and pharmacokinetic profiles of LAAM when administered by the intravenous and the oral routes to opioid-experienced human volunteers. The objectives were 1) to characterize the pharmacodynamic profile including the time to onset, duration of action and magnitude of effects and 2) to characterize the pharmacokinetic disposition of LAAM and its metabolites in plasma after administration by the oral and intravenous routes.
| |
Methods |
|---|
|
Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
Subjects
The participants were healthy adult male volunteers recruited
through newspaper advertisements and word of mouth. All volunteers were
current intravenous users of opiates, but were not physically dependent
on opioids or on any drugs except nicotine and currently were not
seeking treatment for substance abuse or dependence. Physical
dependence was assessed by interview and examination, and by extended
observation in a drug-free environment before study participation.
Volunteers received a medical screening examination which included
hematology, blood chemistries, urinalysis, assessment for adequate
venous access and an electrocardiogram. Psychological assessments were
conducted with the Structured Clinical Interview (SCID-II) (Spitzer and
Williams, 1986), and subjects diagnosed with any Axis I disorder other
than substance abuse or dependence were excluded.
Nine subjects were enrolled in the study, but three were discharged before completion of the study. One was discharged after experiencing a wheal and flare reaction at the site of intravenous infusion of LAAM, and two were discharged because their self-reports were inconsistent with observable signs of drug effects. Six subjects completed the study. All were black males, age 28 to 46 years (mean, 37.3 years). They reported an average of 12 years education (range, 11-14 years). All subjects met the DSM-III-R diagnostic criteria for an opiate use disorder (n = 5 for dependence; n = 1 for abuse) and for cocaine dependence. The group reported an average of 16.7 years of heroin use (range, 4-28) and reported using heroin approximately 15 of the past 30 days (range, 6-26). This study was approved by the local Institutional Review Board; subjects gave their written informed consent and were paid for their participation.
Setting/General Procedure
The study was completed while subjects resided on a closed
14-bed research unit that was described previously (Walsh et
al., 1995). This facility is staffed by licensed nursing personnel 24 hr/day and is used exclusively for behavioral pharmacology research.
Subjects were required to adhere to written program rules and protocol
restrictions (i.e., dietary, sleep hours, etc.). Recreational activities were provided including exercise equipment, arts and crafts projects, television and video games. Urine specimens were collected daily and randomly tested for evidence of illicit drugs
on an EMIT system (Behring Diagnostics, San Jose, CA) and/or using
thin-layer chromatography to ensure the absence of drugs other than
those administered experimentally. Breath alcohol tests also were given
to the subjects on admission and at weekly intervals. Breathalyzer
tests were negative for alcohol, and no illicit drug use was found in
any subject during the study. Subjects were maintained on a
caffeine-free diet. Five of the six subjects were cigarette smokers;
they were allowed free access to cigarettes except for during and 1 hr
preceding each experimental session.
Experimental Design
All subjects received a single screening dose of LAAM (10 mg) given intravenously during the first week of the study. The purpose of this screening dose was to assess for any idiosyncratic reaction to the intravenous infusion or for unusual sensitivity to LAAM. This drug administration was single-blind, plasma samples were not collected and data from this session were not included in any analyses.
A double-blind, double-dummy crossover design was used to evaluate the effects of oral and intravenous LAAM. For the double-dummy control, subjects received both an oral and an intravenous preparation on each study day, but staff and subject were unaware of which, if either, was active. The oral solution was administered immediately before the intravenous solution. Subjects were tested once weekly with one of the following doses: placebo, oral LAAM (20 and 40 mg/70 kg b.wt.) and intravenous LAAM (20 and 40 mg/70 kg). There were at least 7 days between each experimental session. Doses were administered with a constrained randomized order; the constraint was that administration of the lower intravenous dose always preceded the higher intravenous dose. Subjects, nursing staff and technical staff involved in data collection were blind to the dosing schedule.
Drugs
An oral LAAM HCl solution was obtained from the Research Triangle Institute through the Chemistry and Pharmaceutics Branch, National Institute on Drug Abuse (Rockville, MD). The stock solution was a 10 mg/ml concentration. All oral LAAM doses were prepared by adding an additional volume of a sugar- and alcohol-free flavored syrup (Ora-Sweet SF, Paddock Laboratories, Inc., Minneapolis, MN) diluted with water (1:4) that contained 12 ng/ml denatonium benzoate (Bitrex, JH Walker and Company, Inc., Mt. Vernon, NY) as a bitter taste-mask for a final dose volume of 20 ml. The same volume of diluted Ora-Sweet solution with Bitrex served as the oral placebo solution.
Intravenous solutions of LAAM HCl were prepared from bulk powder manufactured through Orpharm, Inc. (Houston, TX) and supplied through BioDevelopment Corporation (McLean, VA). LAAM HCl was weighed and dissolved in the appropriate amount of sterile water for injection (Abbott Laboratories, North Chicago, IL) for a total delivery volume of 2 ml. Solutions were prepared aseptically under a laminar flow hood and filtered through a 0.22-µm-pore-size filter (Millipore Products Division, Bedford, MA) into a sterile pyrogen-free vial. Placebo infusions consisted of saline for injection USP (Fjisawa USA, Inc., Deerfield, IL). All intravenous doses were in a volume of 2 ml delivered through a venous catheter over 1 min by a staff physician.
Experimental Sessions
Subjects were fasted from midnight preceding each of the five experimental sessions. Intravenous catheters were inserted into each arm within an hour before the start of the session; one was used for drug administration and the other for collection of blood samples. A slow-drip intravenous line was kept in place during the experimental session only. The subjects were escorted from the residential unit to the experimental session room at approximately 8:30 A.M. The subject was seated in a cushioned chair directly in front of a Macintosh computer which was used to collect data. The computer recorded physiological measures (except pupil diameter) and presented all questionnaires in the appropriate order. Physiological measures (except for pupil diameter) were collected by an automatic physiologic monitor (Noninvasive Patient Monitor model 506, Criticare Systems, Waukesha, WI) that was interfaced with the computer. Subjects entered their questionnaire responses by use of a keyboard. A research assistant, who was blind to the treatment, was seated behind the computer with a keyboard available to initiate tasks and to enter observer-rated measures. Data printouts were collected after each session, and the data were transferred electronically to spreadsheets for analyses.
Physiological measures. The subjects were monitored continuously throughout each session. Data collection began 30 min before drug administration and continued for 8 hr after drug administration. Oxygen saturation, heart rate, skin temperature and systolic and diastolic pressure were collected every 3 min during the session. Pupil diameter was determined from photographs taken in constant ambient room lighting using a Polaroid camera (Polaroid Corp., Cambridge, MA) with a 2× magnification; photos were taken at 30 min before, at 5 and 15 min after drug administration and at 15-min intervals thereafter for the duration of the 8-hr session. Respiratory rate was measured manually by counting the number of breaths per minute at baseline and once every 15 min throughout the 8-hr session.
Subject-rated measures.
During the experimental sessions,
subjects responded to three computerized questionnaires: the Visual
Analog Questionnaire, the Adjective Rating Questionnaire and the short
form of the Addiction Research Center Inventory (Martin et
al., 1971). For the Visual Analog Questionnaire, the subject rated
"Do you feel any DRUG EFFECT?," "How HIGH are you?," "Does
the drug have any GOOD EFFECTS?," "Does the drug have any BAD
EFFECTS?," "Do you LIKE the drug?," "Does the drug make you
feel SICK?," and "How much do you desire OPIATES now?" by
positioning the 1-mm cursor along a 100-point line marked at either end
with "not at all" or "extremely." These seven visual analogs
were rated 30 min before, 5 and 15 min after drug administration and at
15-min intervals thereafter for the duration of the session.
). The ARCI and adjective rating scales were completed 30 min before and at 30-min intervals after drug administration for the
duration of the 8-hr session.
Observer-rated measures. Observer ratings were completed by a research assistant who rated the subject on a 5-point scale from 0 (not at all) to 4 (extremely) with the same adjective rating list that the subjects completed. Observers made their ratings based on observation and on spontaneous comments by the subjects. Observer ratings were completed 30 min before and at 30-min intervals after drug administration for the duration of the 8-hr session.
Post-session measures. Several measures were collected periodically for up to 4 days after completion of each experimental session. Data collection was conducted by nursing personnel on the residential unit, and all questionnaires were computerized. Subjects responded on the same Visual Analog Scale and Adjective Rating Scale described above. Nursing personnel rated subjects for opiate effects with the same Adjective Rating Scale and obtained pupil photographs. Each of these measures was collected at 9, 12, 36, 48, 60, 72 and 96 hr after drug administration.
Pharmacokinetic Analysis of LAAM in Plasma
Blood samples were collected 30 min before and at 1, 5, 15, 30 and 45 min, and 1, 1.5, 2, 2.5, 3, 4, 5, 6, 9, 12, 36, 48, 60, 72 and
96 hr after drug administration. Approximately 8 ml of blood was drawn
through an intravenous catheter in the antecubital vein on the arm
opposite the one where the intravenous infusion was administered.
Samples were drawn into a heparinized vacutainer and immediately
centrifuged at 3000 rpm for 10 min. The plasma was removed and frozen
at 
30°C until the time of assay. Samples were assayed by the Center
for Human Toxicology, Salt Lake City, UT for concentrations of LAAM,
nor-LAAM and dinor-LAAM by a gas chromatography/positive ion chemical
ionization-mass spectrometric method that has been described previously
(Moody et al., 1995). The lower limit of sensitivity for the
assay was <5 ng/ml.
Pharmacokinetic parameters of LAAM, nor-LAAM and dinor-LAAM were
obtained by use of model-independent methods (Gibaldi and Perrier,
1982). The plasma AUC was calculated by the trapezoidal rule from 0 to
96 hr after dose administration [AUC (0-96)]. The elimination rate
constant (
z) was estimated by linear
regression of the last 3 to 4 plasma concentration data points of the
terminal postdistribution phase. The terminal half-life
(T1/2) was estimated from
0.693/z. The AUC (
) was calculated as
follows: AUC () = AUC (0-96) + Ct/z, in which
Ct represents the last point plasma concentration. The apparent total body clearance (CL) of LAAM was
calculated according to the formula: CL = dose/AUC.
The apparent oral total body clearances of nor-LAAM and dinor-LAAM were
calculated as the product of CL/F and F where
F is the fraction of the dose absorbed. Mean residence time
was calculated as the ratio of the area under the first moment curve
extrapolated to infinity to AUC(). Cmax
and Tmax are the peak plasma concentrations and time-to-peak concentrations observed rather than calculated, respectively. The observed absolute bioavailability of LAAM
(Fobs) was determined according to the
relationship: Fobs = (AUCoral/AUCi.v.) × (dosei.v./doseoral).
Data Analysis
The time-course data served as the primary analyses for all dependent measures except for the plasma data. Time-course data were analyzed by two-factor ANOVA (drug condition × time). For all measures collected during the experimental sessions, time course was analyzed for the 8 hr after drug administration. Physiological data collected on-line during the session (i.e., heart rate, blood pressure, skin temperature and oxygen saturation) initially were summarized into 15-min averages for each subject (one interval at base- line and 32 intervals after drug administration), thus corresponding with the schedule of data collection for respiratory rate, pupil diameter and questionnaires. Measures that were collected during the experimental session and on the residential unit were analyzed as time course up to 96 hr after drug administration (including visual analogs, subject- and observer-rated adjectives, pupil diameter and plasma).
Further analyses were conducted with AUC and peak minimum and maximum
scores where appropriate by one-factor ANOVA. Results were generally
consistent with the outcome for main effects of LAAM condition from the
time-course analysis, and therefore, are reported only when the results
between the analyses differ. To determine the time required for the
peak response to occur, the time at which the peak difference score
from baseline (either an increase or decrease) was determined for each
individual subject and these scores were then averaged across the
group. "Time-to-peak" data were generated from the 96-hr time
course when available and from the 8-hr time course for those measures
collected only during the experimental session. These data were
analyzed by one-factor ANOVA. For all analyses, significant main and
interaction effects were evaluated further by use of post hoc tests,
including ANOVA and/or Tukey's tests where appropriate. All repeated
measures data were adjusted for sphericity by Huynh-Feldt corrections. Statistical significance was indicated when P 
.05.
| |
Results |
|---|
|
Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
Pharmacodynamic Effects of LAAM
Onset of pharmacological action. Data shown in figure 1 represent the early portion of the time-action curve (i.e., the first 3 hr after drug administration) and are used to illustrate the initial response to oral and intravenous LAAM administration. Scores on two representative visual analog measures, "any drug effect" and "liking," are shown (upper and middle panels). The magnitude of effects on these measures was dose-related for LAAM regardless of whether the drug was administered orally or intravenously. Statistical comparisons (see table 1) revealed that for the measure "any drug effect," scores after LAAM given intravenously were elevated significantly above baseline within 5 min after administration of both the 20- and 40-mg doses (P < .05; Tukey's test). In contrast, the effects of LAAM given orally appeared more slowly. Oral LAAM at 40 mg produced significant score elevations by 2.5 to 3.0 hr for these measures; whereas the low dose of oral LAAM (20 mg) failed to produce significant score elevations on any of the visual analog measures throughout the full 96-hr time course. The profile of LAAM effects shown in figure 1 is similar to that obtained for the visual analog measures of "high" and "good effects" (table 1). LAAM did not significantly alter ratings of "bad effects," "feel sick" or "desire for opiates."
|
|
Profile, magnitude and duration of action. Subjective and observer-rated measures. The subjective effects of LAAM generally were dose related regardless of the route of administration; however, in most cases the 20-mg dose of oral LAAM did not produce significant elevations on subjective indices of opioid effects. As described above, both intravenous doses (20 and 40 mg) and 40 mg of oral LAAM significantly increased visual analog ratings of positive drug effects including "any drug effect," "liking," "high" and "good effects." Data collected during the full 96-hr time course for the measure "How high are you?" are shown in figure 2 (upper panel); these data generally are illustrative of the time-action and dose-response profiles obtained for LAAM. As can be seen, the overall magnitude of the subjective response to intravenous LAAM was greater when compared with responses after administration of the identical oral dose of LAAM during the early portion of the time-action curve. Thus, the response to 40 mg intravenous LAAM was statistically greater than the response to 40 mg oral LAAM for approximately the first 2 hr after drug administration (Tukey's test; P < .05); the same pattern was found for the 20-mg intravenous and oral doses and these differences were apparent for up to approximately 9 hr. During the latter portion of the time course when the effects of LAAM were beginning to decline (i.e., after approximately 9 hr), the magnitude of LAAM effects were generally comparable across the two routes. Despite the noticeable differences in the magnitude of drug effects during the early portion of the time-action curves produced by intravenous and oral LAAM, comparison of the AUC values which include both duration and magnitude of effects did not reveal any statistically significant differences between equal doses of LAAM given orally versus intravenously.
|
.05), whereas marginal increases were observed on ratings of itchy skin
and heavy/sluggish feeling (P < .10). Each of these items are
descriptive of prototypic opioid agonist effects. Scores on the
composite Fraser scale, also sensitive to opioid agonist effects, were
elevated significantly by all active doses of LAAM in comparison
with placebo (Tukey's test, P < .05). The results for the
observer-rated adjective checklists were remarkably similar to those
obtained from the subjects (table 1). Observers rated significant
increases after administration of LAAM in comparison with placebo on
the following measures: nodding; skin itchy; heavy/sluggish feeling;
dry mouth; good mood; and sleepy. Observers rated significant increases
on at least one of these prototypic opioid agonist items after
administration of all active doses of LAAM; however, these effects were
more pronounced for the high dose (40 mg) than the low dose (20 mg)
regardless of whether the drug was administered intravenously or
orally. The observer ratings were also sensitive to the difference in
latency to onset of drug effect for the two routes of administration.
For example, ratings of "itchy skin" were elevated significantly
within 1.5 hr of administration of 40 mg of intravenous LAAM in
contrast to 3.5 hr for the same dose given orally (Tukey's test;
P .05).
LAAM did not significantly alter any of the ARCI subscales during the
8-hr experimental session. There was a nonsignificant trend (P = .061) for scores on the PCAG-Sedation Scale to increase during the
active dose sessions. There were also significant main effects of time
for the PCAG and the BENZ scales (F[16,80] = 2.94 and
2.36, respectively; P < .05), whereby the PCAG scores increased and the BENZ scores decreased as a function of time in session.
Physiological measures. Pupillary response proved to be the
most sensitive physiological index of LAAM action under these dosing
conditions, and therefore, these data are used to describe the
time-action and dose-response effects of LAAM. Data for pupil diameter
are shown for the full 96-hr time course in the lower panel of figure
2. As already described, intravenous LAAM produced miosis more rapidly
than oral LAAM. For intravenous LAAM, the degree of pupil constriction
was dose-related; the low dose (20 mg) produced less constriction than
the high dose (40 mg). The duration of action was also related to dose,
with significant miosis persisting for 36 hr after 20 mg but 72 hr
after 40 mg (Tukey's test; P .05). In contrast to the failure
of oral LAAM at 20 mg to produce any appreciable subjective effects,
this dose produced significant pupillary constriction, relative to base line, within 2.5 hr, which persisted for 48 hr after dosing (Tukey's test; P .05). LAAM, 40 mg given orally, produced significant pupillary constriction from 2 to 60 hr after dosing. Despite the observable differences for rate of onset and decline of miosis, analysis of the AUC values for pupil diameter did not reveal
significant post hoc differences between the two routes of
administration or between LAAM doses.
LAAM produced few other pronounced physiological effects when
administered across this dose range. LAAM did not produce large or
clinically significant reductions in oxygen saturation. The main effect
of LAAM dose on oxygen saturation failed to reach significance (P = .055), whereas there was a significant LAAM dose × time
interaction on oxygen saturation (table 1). However, the maximum
observed decline in oxygen saturation was less than 2% after any
active LAAM dose. No significant effects of LAAM were observed on
respiratory rate.
Analysis of the 8-hr time course revealed that LAAM did not
significantly alter heart rate or systolic or diastolic blood pressure.
Analysis of the peak responses (minimum or maximum) confirmed the
findings for physiological measures with one exception. Compared with
placebo, heart rate was decreased significantly by active LAAM doses
when assessing the maximum decrease for the session (F(4,
20) = 5.01; P = .009), with the greatest decrease (7 bpm)
occurring after administration of 40 mg intravenous LAAM (Tukey's
test; P < .05). LAAM produced a main effect on skin temperature as well as a dose × time interaction (table 1). These resulted from the tendency for active LAAM doses to increase skin temperature modestly in contrast to the decline in skin temperature observed during
the course of the 8-hr session after placebo administration.
Pharmacokinetic Profile
Plasma concentrations of LAAM and its metabolites, nor-LAAM and
dinor-LAAM, were measured throughout the 96-hr time course after
dosing. Figure 3 illustrates the
concentrations of the parent drug, LAAM, after administration by the
oral and intravenous routes at 20 mg (left panel) and 40 mg (right
panel). Concentrations of LAAM in plasma increased with dose regardless
of route of administration; however, these increases were not
dose-proportional. For example, the differences in the AUC values for
LAAM when comparing the 20-mg dose with the 40-mg dose were
approximately 2.5- and 2.4-fold greater for intravenous and oral
administration, respectively (table 2).
Moreover, LAAM clearance and half-life are increased at the higher dose
for both the oral and intravenous conditions. Together these data
suggest a trend toward nonlinear kinetics for LAAM itself, although
linearity cannot be assessed accurately with these data because only
two active doses were administered. Statistical comparison of LAAM
clearance and half-life values for the 20 and 40 mg doses revealed no
significant dose-related differences on these parameters (P > .05; paired sample two-tailed t tests), although power is
limited to detect a difference with the small sample size. The
estimated half-life of LAAM was excluded from the analysis for one
subject because it was determined to be an outlier according to
Dixon's test (r01 = 0.82; P < .005; Dixon, 1951). The estimated half-life for this subject (125 hr) resulted from the plasma values over the latest portion of the time-action curve (i.e., 48- 96 hr) showing a relatively
flat function with limited decline.
|
|
Intravenous administration of LAAM led to significantly higher peak concentrations of LAAM (Cmax) than oral administration for both the 20- and 40-mg doses; the Cmax values were approximately 5- and 12-fold higher for intravenous LAAM at 20 mg and 40 mg, respectively (table 2). LAAM was distributed rapidly after intravenous administration as evidenced by the rapid peak and decline in the first 5 min after infusion. The time frame in which LAAM could be detected in plasma was dose related; LAAM was detectable in plasma for 36 hr and 72 hr after administration of the 20- and 40-mg doses, respectively. Bioavailability estimates generated from comparison of the intravenous and oral dose conditions suggest that the parent drug LAAM has an oral bioavailability of approximately 47 to 48% (table 2).
The concentrations of the two metabolites, nor-LAAM (upper panel) and
dinor-LAAM (lower panel), are shown in figure
4. These data are shown on a log scale
ranging to 100 ng/ml in contrast to the scale for LAAM concentrations
shown in figure 3, which ranges up to 1000 ng/ml. The sequential nature
of the metabolic path (i.e., LAAM
nor-LAAM dinor-LAAM) is evidenced by 1) the time-ordered appearance of LAAM,
nor-LAAM and then dinor-LAAM, respectively, in plasma under all dosing
conditions; 2) the time-ordered Tmax values
describing the time required to reach peak plasma concentration (table
2); and 3) the sequential disappearance from plasma of LAAM, nor-LAAM
and dinor-LAAM (see figs. 3 and 4). Administration of LAAM by the oral
route reliably produced higher concentrations of nor-LAAM and
dinor-LAAM than intravenous administration for both LAAM doses from
approximately 2 to 24 hr after drug administration (see fig. 4).
However, AUC values differed across routes only for the 20-mg dose of
LAAM and were similar after administration of the 40-mg dose (see table
2). Both metabolites were present in plasma at 96 hr after a single intravenous or oral dose of 40 mg; their long duration of action is
also apparent from the calculated T1/2
values which ranged from 24 to 38 hr for nor-LAAM and from 66 to 90 hr
for dinor-LAAM (see table 2). Residual dinor-LAAM was detected 1 week
after LAAM administration on three single occasions as illustrated by the modest baseline elevations for dinor-LAAM shown in figure 4.
|
Side Effects
Although there was no significant main effect of LAAM condition on the visual analog measure "Does the drug make you feel sick?," there was a significant effect of time (F[41,205] = 2.95; P = .021). Post hoc analyses revealed that the 40-mg dose of LAAM given both orally and intravenously significantly increased ratings of "sick" compared with placebo during the latter portion of the time course (i.e., between 12 and 24 hr after dosing). Moreover, review of the medical charts revealed that vomiting occurred in response to LAAM administration in at least half of the subjects after administration of LAAM at 20 and 40 mg p.o. and 40 mg i.v. at some point during the 96 hr after acute dosing.
| |
Discussion |
|---|
|
Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
This study demonstrates that intravenous administration of LAAM
produces pronounced subjective and physiological effects in humans that
appear almost immediately after infusion and more rapidly than those
produced by LAAM given orally. The pharmacokinetic analyses reveal that
these effects appear at a time when LAAM, but not its active
metabolites nor-LAAM and dinor-LAAM, are detected in plasma. These data
suggest that the parent drug is primarily responsible for producing
these immediate effects, and thus, LAAM is pharmacologically active in
humans when administered parenterally and should not be characterized
as merely a prodrug. These findings are in contrast to current beliefs
that arose primarily from two previous clinical studies that reported
an unusually slow onset for the effects of intravenous and subcutaneous
LAAM in comparison with oral LAAM (Fraser and Isbell, 1952; Fraser
et al., 1954), but are in agreement with several preclinical
studies that have reported a shorter latency of onset for parenteral
LAAM effects (e.g., Henderson, 1976a, 1976c; Archer, 1976).
Consistent with the classification of LAAM as a pure mu
agonist, the profile of effects produced by LAAM in the present study was mu agonist-like. LAAM produced significant pupillary
constriction, and elevated subject-rated and observer-rated scores on
an array of global measures of euphoric effects (e.g.,
"high" and "liking" for the drug) as well as prototypic opioid
agonist effects (e.g., itchy skin and nodding). The
magnitude of these effects was generally dose dependent regardless of
the route of administration. The response to intravenous LAAM occurred
within 5 min of infusion in all subjects; significant miosis and
elevations of subjective ratings of drug effect and euphoric effects
were immediately apparent, whereas the peak effects were substantially
delayed and occurred within 4 to 5 hr after infusion. In contrast, the
effects of LAAM given orally appeared within 1 to 2 hr after dosing and
continued to rise, peaking between 8 and 12 hr after dosing, depending
on the measure (see fig. 2). This time-action profile for oral LAAM is
consistent with previous studies that have characterized the response
to acute doses of oral LAAM in dogs (Henderson, 1976c), monkeys
(Henderson, 1976a, b) and humans (Fraser and Isbell, 1952; Irwin
et al., 1976; see also Sollod and Goldstein, 1976). Although the onset of intravenous LAAM effects was faster than that of oral
LAAM, no statistical between-route pharmacodynamic differences were
found for the calculated peak responses and AUC values obtained for a
given dose (e.g., 20-mg oral compared with 20-mg
intravenous), which suggests no overall differences in the magnitude of
the pharmacodynamic effects between the two routes of administration.
Our findings on the immediate response to intravenous LAAM are in
direct contrast to those of the early parametric study published by
Fraser and Isbell (1952). Although it is impossible to reconcile the
results of these studies retrospectively, it is plausible that specific
methodological differences contributed to these contradictory findings,
including the 1) dose ranges, 2) dependent measures and 3) subject
populations. In the early study, intravenous LAAM was evaluated across
a range of test doses (i.e., 10-30 mg) that was somewhat
lower than tested in the present study (i.e., 20-40 mg).
Given a relative potency estimate ratio of 1:1.2 of methadone/LAAM, the
highest test doses in these studies (30 and 40 mg) are approximately
equivalent to oral doses of 25 and 33 mg of methadone, respectively.
These doses may, in fact, be fairly low when one considers that
participants in both studies were experienced opioid users with some
level of opioid tolerance. This suggestion is supported by findings in
the present study that oral LAAM at 20 mg failed to produce any
significant subjective effects and oral and i.v. LAAM at 40 mg failed
to alter some indices typically sensitive to opioids, including the
ARCI, adjective composite scales and respiration (e.g.,
Jasinski and Preston, 1986; Walsh et al., 1994; Zacny
et al., 1994). The earlier study relied solely on clinical
observation techniques rather than the controlled physiological and
self-report measures used in the present study. Finally, although
limited detail is provided regarding the drug histories of participants
in the Fraser and Isbell study, it is stated that patients had a recent
history of morphine addiction but were withdrawn at the time of the
study, a standard practice in early opioid studies at the Lexington
Addiction Research Center. It is possible, therefore, that their study
population may have been more tolerant than our nondependent sporadic
opioid abusers. Thus, it is plausible that administration of relatively
low LAAM doses to opioid-tolerant individuals coupled with sole
reliance on observational measures may have occluded the detection of
drug effects in this earlier study. Fraser and Isbell reported that intravenous LAAM produced measurable effects by 4 to 6 hr after drug
administration; this time frame corresponds with the time when the peak
subjective responses to intravenous LAAM were observed in the present
study.
Another difference between the present study and the earlier study is
that the subjects in the present study were all African American,
whereas the subjects in the Lexington study were all Caucasian. This
potentially could be important if there are significant racial
differences in sensitivity to or metabolism of LAAM. It is well known
that certain enzyme systems involved in drug metabolism, such as P450
2D6, exhibit genetic polymorphisms that can lead to significant
interindividual metabolic differences. LAAM is metabolized primarily
through N-demethylation to its active metabolites (e.g.,
Kaiko and Inturrisi, 1975; Chiang et al., 1995), and recent data from in vitro human liver metabolic studies suggest
that cytochrome P450 3A4 is the enzyme primarily involved in the
production of nor-LAAM and dinor-LAAM (Moody et al., 1997).
Although there is no current evidence supporting the existence of
polymorphic forms of P450 3A4 (Wilkinson, 1996), the possibility of
genetic variants cannot be ruled out and neither can the participation of other P450 enzymes in the metabolism of LAAM. Thus, although existing evidence does not support the argument that significant metabolic differences exist or that other critical pharmacokinetic or
neurochemical factors vary across these two racial groups, the
potential influence of such differences cannot be excluded as factors
contributing to the differential outcome of these two studies.
Consistent with previous studies, these data indicate that LAAM is
extraordinarily long acting and produces measurable pharmacodynamic effects for 48 to 60 hr after a single dose. The duration of action was
dose related, with larger doses producing more sustained effects than
lower doses, and was equivalent after intravenous and oral administration. The calculated half-life estimates ranged from 14 to 37 hr for LAAM, and 24 to 38 hr for nor-LAAM with some variability caused
by individual differences, as well as dose and route differences (see
table 2). These values are generally within the range of previous
estimates (Billings et al., 1973; Chiang et al.,
1995). The estimated half-life for dinor-LAAM ranged from 66 to 89 hr across conditions; although these values are also similar to previous reports (Chiang et al., 1995), the sampling period was
equivalent to roughly only one half-life and the calculations required
more extrapolation than desirable for an accurate estimate.
Previous studies have attempted to correlate the time-action profile of
LAAM with the presence of LAAM and its metabolites in plasma to
identify the compound that best accounts for the pharmacodynamic
effects. The present data suggest that all three drugs are active and
contribute to the pharmacological activity of LAAM. During the earliest
portion of the time-action curve for intravenous LAAM, it is evident
that the parent drug is active and producing significant subjective and
physiological effects. Pronounced pharmacodynamic effects were observed
within 5 min of infusion and LAAM was detected in all subjects during
this same period. In contrast, nor-LAAM was detected in only one
subject during this early portion of the time curve and was not
detected in the other subjects until approximately 45 min
postinjection. For all dynamic measures, the effects continued to rise
after concentrations of the parent drug had already begun to decline, and concentrations of nor-LAAM and dinor-LAAM were still rising. It is
important to note that nor-LAAM has been characterized in preclinical
and clinical studies as being substantially more potent than both LAAM
and dinor-LAAM (Lukas et al., 1980; Perez-Reyes, 1985;
Nickander et al., 1974; Smits, 1974). After all active LAAM doses, dinor-LAAM was still present in plasma at 96 hr after drug administration and showed little sign of decline, yet no residual drug
effects were detected at this time under any condition, which suggests
the possibility of acute tolerance. Thus, comparison of the time to
reach peak effect for miosis and subjective measures (e.g.,
ratings of "high" or "drug effect") with peak plasma
concentrations of drug (see table 2) suggests that the time course for
concentrations of nor-LAAM corresponds most closely with the dynamic
effects of the drug and this is consistent with other reports
(Henderson, 1976a; Henderson et al., 1977c; Perez-Reyes,
1985). The pharmacodynamic effects of LAAM produced by a given dose
(e.g., 40 mg) were generally equivalent in magnitude across
the time-action curve (i.e., AUC values) regardless of the
route of administration; this is surprising in light of the finding
that much higher concentrations of the parent drug, LAAM, were achieved
by intravenous administration whereas greater nor-LAAM concentrations
were achieved by oral administration.
The pharmacokinetic profile of LAAM observed in the present study is
complex but consistent with previous reports collected from laboratory
animals and humans. After intravenous administration, there was an
immediate rise in LAAM concentrations in plasma that peaked between 1 and 5 min after infusion and fell rapidly (e.g., 0-550
ng/ml during 5 min declining to 200 ng/ml at 10 min after 40 mg). This
sharp decline suggests that the drug is distributed rapidly to other
compartments where it may remain sequestered for some duration given
its highly lipophilic character. This rapid peak and distribution is
similar to the pharmacokinetic profile of intravenous LAAM when given
to both monkeys (Misra and Mule, 1975) and rats (Henderson et
al., 1977a). In contrast to i.v. administration, peak
concentrations of LAAM were not achieved until 2.5 hr after oral
administration of the drug. This time course is also consistent with
preclinical and clinical pharmacokinetic studies of oral LAAM dosing
(Billings et al., 1974; Henderson et al., 1977b,
c; Kaiko and Inturrisi, 1975; Chiang et al., 1995). These
present data suggest that the kinetic properties of LAAM may be
nonlinear; AUC values increased in a greater than dose-proportional fashion and there was an accompanying trend for clearance and half-life
to increase with increasing dose. Although these differences did not
achieve statistical significance, a fuller dose-effect evaluation will
be required to characterize and model the pharmacokinetic profile of
LAAM.
The maximum plasma concentration (i.e.,
Cmax) of LAAM achieved after intravenous
administration was roughly 5.5- and 12-fold greater than for oral LAAM
at 20 and 40 mg, respectively. This is consistent with another study
that evaluated the pharmacokinetics of LAAM in monkeys and found lower
peak levels of free parent drug after oral versus parenteral
(i.e., subcutaneous) LAAM (Misra and Mule, 1975). Despite
the large differences observed in initial circulating concentrations of
parent compound in this study, subsequent peak and AUC
concentrations of nor-LAAM and dinor-LAAM were roughly equivalent
between the routes or even higher after oral compared with intravenous
dosing. This is not necessarily unexpected because the oral dose, but
not the intravenous dose, can be subjected to first-pass metabolism
potentially leading to greater biotransformation to the active
metabolites. A large first-pass effect for oral LAAM is supported by
the finding in the present study that the bioavailability estimates for
oral LAAM were less than 50%. Although no previous controlled
comparisons of intravenous and oral LAAM in humans were found in the
literature, a preclinical study conducted in rats reported similar
results estimating the oral bioavailability of LAAM to be approximately
60% (Henderson et al., 1977a). The pharmacokinetic
profile for LAAM under these acute dose conditions is likely to be
dissimilar to that observed during chronic LAAM administration. Because
the active metabolites tend to accumulate with repeated dosing
(Billings et al., 1974), it would be expected that the
parent/metabolite ratio would decrease under chronic dosing conditions.
In summary, the present results indicate that LAAM administered intravenously produces opioid agonist effects that appear immediately after infusion; this finding is in contrast to previous clinical studies that reported a delayed onset of action for parenteral LAAM. The immediate onset of action after intravenous LAAM is primarily attributable to the pharmacological activity of the parent drug, rather than the demethylated metabolites, which indicates that LAAM is not merely an inactive prodrug. LAAM given orally and intravenously was equieffective in producing a constellation of prototypic opioid agonist effects of long duration, although the relative contributions of the parent drug and metabolites to these pharmacodynamic actions varied across the two routes of administration. These data suggest that LAAM possesses abuse potential; the gradual onset of effects after oral administration is likely to minimize the risk of abuse by the oral route. However, the slow onset of effects produced by the metabolites after oral dosing justifies the labeling recommendations to warn patients that toxicity may result if other drugs are taken after LAAM administration. The rapid onset of effects after intravenous LAAM indicates that the risk for abuse and diversion to the parenteral route may be substantially greater than previously believed. Because the commercially available product is formulated as a clear concentrated aqueous solution that could be injected easily, these data suggest that care should be exercised in the preparation of clinical doses to dilute the concentrate in a vehicle with physical properties that will deter parenteral use.
| |
Acknowledgments |
|---|
The authors thank Jane Garner, Shirley Podgurski, L.P.N., Veronica Beverly, and John Yingling for technical services; Iona Johnson for pharmacy services; Mike DiMarino for statistical analyses; and David Ginn, M.D., Ira Liebson, M.D. and the Residential Nursing Staff for medical consultation and supervision. Special thanks to Dr. Nora Chiang and Dr. Betty Tai of the Medications Development Division of the National Institute on Drug Abuse (NIDA) for consultation and for arranging support for the LAAM plasma assays which were conducted at the Center for Human Toxicology, Salt Lake City, UT under NIDA contract no. 271-91-9205 awarded to Dr. Roger Foltz and Dr. David Moody. We are grateful to BioDevelopment Corporation of McLean, VA; Orpharm, Inc. of Houston, TX; and NIDA for supplying powdered LAAM and LAAM in solution for these studies.
| |
Footnotes |
|---|
Accepted for publication December 22, 1997.
Received for publication July 11, 1997.
1 This research was supported by U.S. Public Health Service Research Grants P50 DA 05273 and KO5 DA00050 from the National Institute on Drug Abuse.
2 With the Intramural Research Program of the National Institute on Drug Abuse, National Institutes of Health, Baltimore, MD.
Send reprint requests to: Sharon L. Walsh, Ph.D., BPRU, Behavioral Biology Research Center, Johns Hopkins Bayview Campus, 5510 Nathan Shock Drive, Baltimore, MD 21224-6823.
| |
Abbreviations |
|---|
AUC, area under the curve;
LAAM, l--acetylmethadol;
ARCI, Addiction Research Center
Inventory;
ANOVA, analysis of variance;
BENZ, benzedrine scale;
DSM-III-R, Diagnostic and Statistical Manual of Mental Disorders (3rd
edition, revised);
LSD, lysergic acid diethylamide ("dysphoria"
scale);
MBG, morphine-benzedrine group ("euphoria" scale);
PCAG, pentobarbital-chlorpromazine-alcohol group ("sedation" scale);
S.E.M., standard error of the mean.
| |
References |
|---|
|
Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
-acetylmethadol [LAAM] and active metabolites in plasma following chronic administration.
J Anal Toxicol
1:
1-5.-acetylmethadol (LAAM) after acute and chronic administration.
Clin Pharmacol Ther
21:
16-25[Medline].-acethylmethadol (LAAM), two of its metabolites and morphine and methadone in the rat.
J Pharmacol Exp Ther
215:
382-389-dl-acetylmethadol in the rat: The identification of the probable active metabolite.
J Pharmacol Exp Ther
149:
436-445-Acetylmethadol (LAAM) Pharmacokinetics and metabolism: Current status.
Am J Drug Alcohol Abuse
2:
30-305.-acetylmethadol (LAAM), norLAAM and methadone. Drug
Metab Dispos, in press.-acetylmethadol (LAAM), norLAAM, and dinorLAAM in plasma, urine, and tissue.
J Anal Toxicol
19:
343-351[Medline].-l-Acetylmethdol and its N-demethylated metabolites have potent opiate action in the guinea pig isolated ileum.
Life Sci
14:
2011-2017[Medline].-l-acetylmethadol and two of its metabolites in mice.
Res Commun Chem Pathol Pharmacol
8:
575-578[Medline].
