The Rate of Intravenous Cocaine Administration Determines Susceptibility to Sensitization

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The Journal of Neuroscience, April 15, 2002, 22(8):3244-3250

The Rate of Intravenous Cocaine Administration Determines Susceptibility to Sensitization
Anne-Noël Samaha, Yilin Li, and Terry E. Robinson
Department of Psychology (Biopsychology Program), The University of Michigan, Ann Arbor, Michigan 48109-1109

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The potential for addiction is thought to be greatest when drugs of abuse reach the brain rapidly, because this produces intensesubjective pleasurable effects. However, the ability of drugsto induce forms of cellular plasticity related to behavioral sensitizationmay also contribute to addiction. Therefore, we studied the influenceof rate of intravenous cocaine delivery on its ability to inducepsychomotor sensitization. In one experiment, rotational behaviorin rats with a unilateral 6-hydroxydopamine lesion was used asan index of psychomotor activation, and in a second experiment,locomotor activity in neurologically intact rats was used. Rapid(5-16 sec) intravenous infusions of cocaine induced robust psychomotorsensitization at all doses tested (0.5-2.0 mg/kg). Treatmentsgiven over 25 sec failed to induce sensitization at all dosestested. Treatments given over 50 or 100 sec induced sensitizationonly at the highest dose tested. Thus, the rate of intravenouscocaine delivery has profound effects on the ability of cocaineto induce psychomotor sensitization. This suggests that the temporaldynamics of drug delivery to the brain is a critical factor inthe ability of cocaine to induce forms of neuronal plasticitythat may contribute toaddiction.

Key words: cocaine; psychomotor sensitization; behavioral sensitization; intravenous; rate of infusion; 6-hydroxydopamine lesion; rat

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The rate at which drugs of abuse exert their effects is associated with their abuse liability; thus, drugs, formulations,and routes of administration that yield the most rapid entry ofa drug into the brain are potentially the most addictive (Gossopet al., 1992, 1994; Winger et al., 1992; Hatsukami and Fischman,1996). This is one reason, for example, that smoked cocaine ("crack")is thought to be more addictive than powdered cocaine taken byinsufflation (Hatsukami and Fischman, 1996). Rapid drug deliveryis thought to promote abuse liability because of its influenceon the positive subjective effects of drugs, consistent with reportsthat the positive effects of benzodiazepines (de Wit et al., 1993;Mumford et al., 1995), barbiturates (de Wit et al., 1992), andmethylphenidate (Kollins et al., 1998) are greatest when thesedrugs are administered rapidly. For cocaine, evidence of a relationshipbetween rate of drug delivery and its subjective effects is largelyanecdotal. However, Abreu et al. (2001) recently compared theeffects of a fixed dose of intravenous cocaine delivered over2, 15, or 60 sec and found that rapid rates of infusion producedthe greatest subjective effects (e.g., "high," "liking," and "rush";also see Fischman and Schuster, 1984).

The notion that rapidly administered cocaine not only produces greater subjective effects but also may lead to more avid drug-takingbehavior is supported by studies showing that rapid intravenousdrug delivery is most effective in supporting self-administrationbehavior. With increasing rates of cocaine administration, rhesusmonkeys increase their rate of operant responding and decreaseoperant responding when the rate of administration is decreased(Balster and Schuster, 1973; Panlilio et al., 1998). Primateswill also self-administer lower doses of cocaine if the drug isdelivered more rapidly (Kato et al., 1987). Thus, it appears thatthe reinforcing efficacy of cocaine is greatest when it is administeredrapidly. Furthermore, intravenously administered cocaine is moreeffective in establishing a conditioned place preference thancocaine administered intraperitoneally (Nomikos and Spyraki, 1988).

The subjective pleasurable and reinforcing effects of drugs certainly contribute to addiction, but it is important to rememberthat the transition to compulsive patterns of drug-seeking anddrug-taking behavior is not necessarily a direct function of eithertheir subjective pleasurable effects or their reinforcing efficacy(Robinson and Berridge, 1993, 2000). For example, drug-inducedadaptations in the organization of brain systems that mediatethe incentive motivational effects of drugs may be critical inthe transition to addiction (Lett, 1989; Piazza et al., 1989;Horger et al., 1990; Robinson and Berridge, 1993, 2000). One behavioralmanifestation of this class of drug-induced neuroadaptations isthe phenomenon of psychomotor sensitization (Robinson and Berridge,1993). We hypothesized, therefore, that susceptibility to sensitizationmight be enhanced by the rapid delivery of drugs to the brain.Interestingly, the influence of rate of drug delivery on sensitizationhas never been examined before. We report here that in rats, therate of intravenous cocaine administration has profound effectson its ability to induce psychomotorsensitization.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects
Male Sprague Dawley rats weighing between 200 and 250 gm on arrival were purchased from Harlan Sprague Dawley (Indianapolis,IN). All rats were housed individually in a climate-controlledcolony room maintained on a 14/10 hr light/dark cycle (lightson at 8:00 A.M.).

Experiment 1
Surgical procedures. The purpose of experiment 1 was to investigate the effects of rate of intravenous cocaine delivery onsensitization to the psychomotor activating effects of cocaine,as quantified by measuring rotational behavior in rats with aunilateral lesion of the nigrostriatal dopamine system (Ungerstedtand Arbuthnott, 1970). This particular index of psychomotor activationwas used because it has been shown to be an especially sensitiveindicator of psychomotor sensitization (Robinson, 1984; Crombaget al., 1999).
After 5-9 d of habituation to the animal colony, rats received a unilateral 6-hydroxydopamine (6-OHDA) lesion of the nigrostriataldopamine pathway using procedures described previously (Robinson,1984). Briefly, rats were pretreated with desipramine hydrochloride(15 mg/kg, i.p.) to protect noradrenergic terminals (Breese andTraylor, 1971) and were given atropine methyl nitrate (5 mg/kg,i.p.) before being anesthetized with sodium pentobarbital (52mg/kg, i.p.; The Butler Company, Columbus, OH). Methoxyflurane(Schering-Plough Animal Health Corp., Union, NJ) was used as neededduring surgery to maintain anesthesia. Approximately 30 min afterthe administration of desipramine, a 26 gauge stainless steelinjector was lowered into the medial forebrain bundle and 4 µgof 6-OHDA (dissolved in 8 µl of a 0.9% NaCl/ascorbic acid solution)was infused over an 8 min period at a flow rate of 0.5 µl/min.The injector was left in place an additional 2 min to minimizediffusion upward in the injector tract. One-half of the animalsreceived a lesion in the left hemisphere and one-half receiveda lesion in the righthemisphere.
After 10-14 d of recovery, the development of denervation supersensitivity was assessed by administering apomorphine (0.05mg/kg, s.c., into the nape of the neck) to all rats and measuringcontraversive rotational behavior. At this dose, apomorphine producesmarked circling behavior only if animals are depleted of >90%of the dopaminergic input to the striatum (Marshall and Ungerstedt,1977). The animals were observed 10 min after the apomorphineinjection, and rats that did not meet a screening criterion ofmore than five full rotations in a 1 min period were excludedfrom theexperiment.
After the apomorphine screen, intravenous catheters were implanted in all rats using procedures described previously (Weeks,1972; Crombag et al., 1996). The catheters were constructed fromSILASTIC (Dow-Corning, Midland, MI) tubing [0.30 mm inner diameter(ID), 0.64 mm outer diameter (OD)], two sizes of polyethylene(PE) tubing (0.38 mm ID, 1.09 mm OD and 0.28 mm ID, 0.61 mm OD),and a backport consisting of a 26 gauge piece of stainless steeltubing inserted into a blunted 16 gauge needle affixed to a circularpiece of mesh wire with dental cement (Caine et al., 1993). Briefly,rats were anesthetized with sodium pentobarbital (52 mg/kg, i.p.),and the catheter was placed such that the silicone end was insertedinto the right external jugular vein and the backport exited dorsallybetween the animal's shoulder blades. The catheters were thenflushed with 0.1 ml of gentamicin (50 mg/kg) and 0.1 ml of heparinsolution (30 U/ml, in 0.9% sterile bacteriostatic saline) to preventocclusions and potential microbial buildup in the catheter. Alldrugs were purchased from Sigma (St. Louis, MO) unless otherwisenoted.
After catheter implantation, animals were allowed to recover for 3 d before testing began. During this period and throughoutthe duration of the experiment, catheters were manually flushedonce daily with 0.1 ml of heparin solution. The day before testingbegan, catheters were screened for patency by injecting 0.1 ml(i.v.) of the short-acting barbiturate Pentothal (thiopental sodium,20 mg/ml in sterile water). Rats who failed to become ataxic within5 sec were excluded from the experiment. The same patency testwas performed the day after the drug treatment and on the dayafter the challenge testday.
Apparatus. The test cages consisted of circular plastic buckets 25 cm in diameter and 36 cm in height, the floors of whichwere covered with granulated corncob bedding. Each bucket wasequipped with a photocell-based automated rotometer that recordedquarter, half, and full turns in each direction using an XT-basedpersonal computer (McFarlane et al., 1992). A full turn was definedas four consecutive 90° turns in the same direction. Each ratwas tethered to a homemade liquid swivel (Brown et al., 1976)via a stainless steel cable. The swivel was mounted on a counterbalancedarm allowing the animals to move unhindered in the apparatus.A length of PE20 tubing connected the swivel to a 1.0 ml syringemounted on a Harvard Apparatus (Holliston, MA) syringe pump. Asecond length of PE20 tubing connected the swivel to each animal'scatheter and served as the drug/vehicle infusion line. The pumpswere programmed to infuse a fixed unit dose of 1 mg/kg cocaineover 3 (300 µl/min), 9 (100 µl/min), 16 (50 µl/min), or 34 sec(25 µl/min).

Groups and procedures
Pretreatment phase. After the unilateral 6-OHDA lesion and intravenous catheter implantation, the animals were assigned randomlyto one of six groups. Initially all animals received intravenousinfusions of either saline or 1.0 mg/kg cocaine: four groups receivedcocaine infusions over either 3, 9, 16, or 34 sec, and two controlgroups received saline infusions over 3 or 34 sec, according tothe following procedures. On each test day, the experimenter enteredthe testing room and filled the infusion lines, consisting ofa length of PE20 tubing, with 10 µl of 0.9% NaCl solution or 10µl of cocaine (1.0 mg/kg dissolved in 0.9% NaCl solution). Theremainder of the infusion line was filled with saline solution,which was separated from the drug solution by a small air bubbleto prevent diffusion. The catheters were manually flushed with0.1 ml of heparin to clear potential obstructions before beingplaced in the testing cage, tethered to the liquid swivels viaa lightweight flexible cable, and connected to the drug/salineinfusion lines. A 30 min habituation period followed, during whichtime animals were left undisturbed and baseline levels of rotationalbehavior were monitored in 3 min intervals. The pumps in the testingroom were then activated so that all animals received their injectionsimultaneously, regardless of infusion rate. Each infusion consistedof an initial 17 µl of heparin (volume of the catheter) followedby 10 µl of cocaine or saline followed by an additional 33 µlof heparin. Thus, the total infusion volume was held constantat 60 µl over the four infusion rates. After the infusion, rotationalbehavior was quantified for 21 min in 3 min intervals. After thetest session, animals were disconnected from their tethers andreturned to their home cages. This procedure was repeated for7 consecutivedays.
Withdrawal and cocaine challenge. After the last treatment, animals remained drug-free for 5 d, during which time their catheterswere manually flushed once daily with a heparin solution as describedabove. On day 6 after the last drug/saline treatment, all animalswere tested for the expression of sensitization using the sameprocedures as described above, except that one-half of the animalsin all groups (including animals previously treated with saline)received a challenge intravenous infusion of 1.0 mg/kg cocaineover 3 sec, and the other half received the challenge infusionover 34 sec. One day later, animals previously challenged witha cocaine infusion over 3 sec were now infused over 34 sec, andvice versa. Behavior was recorded for 21 min in 3 min intervalsafter the infusion on each of the 2 challengedays.

Experiment 2
In experiment 1, the influence of rate of infusion on the development of behavioral sensitization to cocaine was examinedin rats with a unilateral 6-OHDA lesion of the nigrostriatal dopaminepathway, using rotational behavior as the index of psychomotoractivation. The purpose of experiment 2 was to investigate thisrelationship in neurologically intact animals, using locomotoractivity as an index of psychomotor activation, as well as toexamine the interaction between dose of cocaine and rate ofinfusion.
Behavioral measures. The locomotor-activating effects of cocaine were measured by placing the animals in the circular testingcages described above, and the same photocell-based automatedrotometers described in experiment 1 were used to record the totalnumber of 90° turns to the left and to the right. This methodessentially divides the circular environment into four quadrants,and total quadrant entries (right/left combined) were used asan index of locomotoractivity.
Surgical procedures. Animals were anesthetized with a mixture of ketamine, xylazine, and acepromazine (77/1.5/1.5 mg/ml, i.p.,at 0.1 ml/100 gm of body weight), and intravenous catheters wereimplanted as described in experiment1.

Groups and procedures
Pretreatment phase. After intravenous catheter implantation, animals were assigned to their respective conditions. All animalsreceived an intravenous infusion of either PBS or 0.5, 1.0, or2.0 mg/kg cocaine in the circular test cages every 3-4 d for atotal of five infusions, using the same procedures as in experiment1. The experimental groups received cocaine infusions over 5 (142µl/min), 25 (27.4 µl/min), 50 (13 µl/min), or 100 sec (6.4 µl/min),and two control groups received vehicle infusions over 5 or 100sec.
Withdrawal and cocaine challenge. Four days after the last treatment, all groups (including animals previously treated withvehicle) received a challenge intravenous infusion of 0.75 mg/kgcocaine over 10 sec to examine the expression ofsensitization.

Rationale for doses and infusion rates
The doses of cocaine used in these experiments (0.5-2.0 mg/kg) were chosen for two reasons. First, they span the range ofintravenous doses previously found to be effective in producingboth psychomotor activation and psychomotor sensitization (Browmanet al., 1998). Second, these doses are within the range oftenused in studies of cocaine self-administration behavior (Sizemoreet al., 1997). The range of infusion times we used (3-100 sec)was chosen because it spans rates (1) often used in studies ofcocaine self-administration behavior and (2) shown previouslyto influence self-administration behavior. For example, in theirstudy on the role of infusion rate on cocaine self-administration,Balster and Schuster (1973) used infusion rates between 5 and100 sec. These rates also span the range shown to influence thesubjective effects of cocaine in humans (Abreu et al., 2001).
In addition, we wanted to study a range of infusion rates that produced different rates of cocaine delivery into the brainbut, importantly, did not differ in the peak brain concentrationsof cocaine achieved. Otherwise, it would be difficult to dissociateeffects attributable to the effective dose achieved versus thoseattributable to the temporal dynamics of cocaine delivery. Thisis the problem in comparing, for example, intravenous and intraperitonealadministrations (Porrino, 1993). The temporal dynamics of cocainedelivery to the brain over the range of conditions used here wereestimated using a pharmacokinetic model developed by Pan et al.(1991). Pan et al. (1991) used microdialysis to measure both theplasma and the brain concentrations of cocaine, given intraperitoneallyor intravenously, to control rats or sensitized rats. They thenestimated the relevant pharmacokinetic parameters by fitting atwo-compartment open model to the data using nonlinear regression.The equations for the model and the parameter estimates are givenin the study by Pan et al. (1991). This model (based on intravenousinfusions) was used to generate the curves shown in Figure 1,using a program provided by Dr. J. B. Justice Jr. (Emory University,Atlanta, GA), with the sampling rate set at 12 points per second(faster rates did not change the curves). Figure 1 shows the estimatedbrain concentrations of cocaine, based on the model, after aninjection of 1.0 mg/kg delivered over 5, 25, 50, or 100 sec (thecurves are the same for 0.5 and 2.0 mg/kg, except for peak levelattained). It is obvious from inspection of Figure 1 that varyingthe rate of infusion between 5 and 100 sec should have no effecton the peak brain concentrations of cocaine. The inset in Figure1 shows an expanded time scale (3 min) to better illustrate theestimated time to achieve half-maximum levels of cocaine in thebrain. The time to half maximum was estimated to vary by approximatelytwofold over the range of doses and infusion rates used here (from43 sec for a 5 sec infusion to 97 sec for a 100 sec infusion).In summary, this pharmacokinetic model suggests that we achievedour goal of spanning a range of infusion rates that produced thesame peak brain levels of cocaine, while yielding different ratesof cocaine delivery to the brain (Fig. 1).

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Figure 1. A pharmacokinetic model developed by Pan et al. (1991) was used to estimate brain concentrations of cocaine (micromolar concentrations) in a 300 gm rat over a 20 min period after an intravenous injection of 1 mg/kg cocaine over 5, 25, 50, or 100 sec (lines from left to right, respectively). The inset shows the same curves, but with the time line expanded to show just the first 3 min. The dashed lines in the inset indicate the time for brain concentrations to reach half maximum after different rates of infusion, based on this model. Note that according to this model, there would be no effect of infusion rate on the maximal brain concentrations of cocaine over the range of conditions used in the experiments reported here. These curves were generously provided by Dr. J. B. Justice Jr, based on the report by Pan et al. (1991) (see Materials and Methods).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1

Figure 2 shows the time course of rotational behavior after the first and seventh infusions of cocaine administered over 3,9, 16, or 34 sec. There was a significant interaction betweentreatment day and rotations in all groups, indicating a significantchange in the behavioral response to cocaine from day 1 to day7 at all infusion rates tested (see figure legends for statistics).Although all groups showed sensitization using this within-subjectsanalysis, it is also obvious from Figure 2 that the change indrug response in animals given cocaine over 34 sec was relativelysmall. Indeed, the rotational response on day 7 was significantlysmaller in animals infused over 34 sec relative to all other groups.

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Figure 2. The mean (±SEM) number of rotations over time (3 min intervals) produced by an intravenous infusion of 1 mg/kg cocaine given over 3 (n = 9), 9 (n = 10), 16 (n = 9), or 34 (n = 9) sec on day 1 and day 7 of treatment. For all treatment conditions, there was a significant increase in the behavioral response to cocaine between days 1 and 7 (two-way ANOVAs; A, main effect of treatment day, F_t(1,16) = 5.35, p = 0.03; treatment day × time interaction, F_i(3,48) = 17.96, p < 0.0001; B, F_t(1,18) = 4.18, p = 0.06; F_i(3,54) = 8.46, p = 0.0001; C, F_t(1,17) = 8.88, p = 0.008; F_i(3,51) = 18.74, p < 0.0001; D, F_t(1,16) = 4.17, p = 0.06; F_i(3,48) = 13.85, p < 0.0001). However, the rotational response on day 7 was significantly smaller in the 34 sec group relative to all other groups (two-way ANOVAs; main effects of rate of infusion, F_(1,15-17) = 7.36-8.11, p < 0.03).

Figure 3 shows the effects of treatment condition on the behavioral response to a 1.0 mg/kg cocaine challenge infusion administeredover 3 or 34 sec. There was no effect of rate of saline infusionon behavior; therefore, the two saline-pretreated groups werepooled to form a single control group. For this between-subjectsanalysis, sensitization is indicated by a response that is greaterthan that in saline-pretreated control animals. Regardless ofthe rate at which the challenge infusion was administered, animalspreviously treated with cocaine infusions over 3, 9, or 16 secshowed a significantly greater locomotor response than saline-treatedcontrols, confirming that these groups were sensitized. Animalstreated repeatedly with cocaine infusions over 34 sec did notdiffer statistically from controls.

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Figure 3. The mean (+SEM) number of rotations (averaged over 12 min) in response to a challenge infusion of 1 mg/kg cocaine administered intravenously over 3 sec (A) or 34 sec (B) in rats pretreated with saline (Sal; n = 8) or 1 mg/kg cocaine over 3 (n = 7), 9 (n = 7), 16 (n = 9), or 34 (n = 7) sec. Animals previously treated with intravenous cocaine infusions over 3, 9, or 16 sec differed significantly from the saline-pretreated control group (one-way ANOVAs followed by Dunnett's tests; $alpha$ = 0.05; A, F₍₄₎ = 8.97, p < 0.0001; B, F₍₄₎ = 9.61, p < 0.0001), but the group given injections over 34 sec did not differ significantly from the vehicle control group (Dunnett's tests). *Different from the saline-pretreated control group (Dunnett's tests).

Experiment 2

Figure 4 shows the locomotor response (quadrant entries), averaged over 15 min after the first intravenous infusion of cocaine,as a function of dose and rate of administration. As in experiment1, there was no effect of rate of vehicle administration on behavior;thus, the two control groups were combined. There was a significantand comparable increase in behavior as a function of increasingdose for all rates of infusion. However, the dose-effect functionin rats given cocaine over 5 sec was shifted to the left relativeto all other groups, which did not differ from one another.

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Figure 4. The mean (±SEM) number of quadrant entries (averaged over 15 min) in response to the first intravenous infusion of cocaine as a function of dose and rate of drug administration (n = 11-13). A significant effect of dose was found at all rates of infusion (two-way ANOVA; main effect of dose: F_(2,133) = 21.42, p < 0.001; main effect of rate of infusion: F_(3,6) = 2.93, p = 0.04; rate of infusion × dose: F_(6,133) = 0.38, p = 0.89). The dose-effect function for the 5 sec condition was shifted to the left relative to all other groups (F_(1,66-67) = 4.71-7.1; p = 0.01-0.04), which did not differ from one another (p > 0.80).

Figure 5 shows the response to a challenge infusion of 0.75 mg/kg cocaine over 10 sec as a function of previous treatmentcondition. Panels on the right show the time course of the locomotorresponse on the day of the challenge test as a function of treatmentcondition. It can be seen that sensitization was characterizedboth by a larger peak response to the drug and by a more rapidonset of the behavioral response. A more rapid onset of drug effectis a hallmark of sensitization (for review, see Segal and Schuckit,1983; Carey and Gui, 1998). Figure 5, A, C, and E, summarizesthese data, illustrating peak drug response (first 6 min). Animalspreviously treated with 0.5 mg/kg cocaine over 5 sec were significantlymore active in response to the challenge infusion than vehicle-treatedcontrols (A), confirming that this group became sensitized. However,animals repeatedly treated with 0.5 mg/kg over 25, 50, or 100sec did not differ significantly from the control group. Similarly,Figure 5C shows that animals previously treated with 1.0 mg/kgcocaine over 5 sec showed an enhanced response to the challengeinfusion relative to controls, whereas animals previously treatedwith 1.0 mg/kg over 25, 50, or 100 sec did not differ significantlyfrom the control group. In contrast, Figure 5E shows that animalsrepeatedly infused with 2.0 mg/kg cocaine over either 5, 50, or100 sec were significantly more active than the control group,indicating that these groups were sensitized. However, animalsrepeatedly infused with this dose of cocaine over 25 sec wereindistinguishable from controls.

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Figure 5. The locomotor response to a challenge infusion of 0.75 mg/kg cocaine over 10 sec as a function of previous treatment condition (n = 6-13). Panels on the right depict the time course of the locomotor response. Left, The mean (±SEM) peak number of quadrant entries (averaged over 6 min) in response to the challenge infusion. Group comparisons were based on the peak values (one-way ANOVAs followed by Dunnett's tests, $alpha$ = 0.05). When previously treated with 0.5 mg/kg, only animals infused over 5 sec differed from the vehicle-treated control group (A, F₍₄₎ = 1.82, p = 0.14, but Dunnett's comparison, p < 0.05). Likewise, in rats treated with 1 mg/kg, only the group infused over 5 sec differed from the control group (B, F₍₄₎ = 3.52, p = 0.01). All groups previously treated with 2 mg/kg (E) differed from the vehicle-treated control group (F₍₄₎ = 3.58; p = 0.01) except those previously infused with this dose over 25 sec (Dunnett's tests). *Different from the saline (Sal)-pretreated control group (Dunnett's tests). Sal, $black-square$ ; 5s, $diamond$ ; 25s, $open circle$ ; 50s, $triangle$ ; 100s, .

Figure 6 shows the same data as Figure 5, but plotted to illustrate the effects of previous cocaine dose on the peak locomotorresponse (first 6 min) at each infusion rate tested. It is clearfrom Figure 6A that when given over 5 sec, all doses tested inducedsensitization. In contrast, when administered over 25 sec, nodose tested induced sensitization (Fig. 6B). When cocaine wasinfused over 50 or 100 sec, there was an approximately linearincrease in the behavioral response to the challenge infusion(Fig. 6, C and D, respectively), although only the groups treatedwith 2.0 mg/kg differed statistically from the control group (i.e.,sensitized). Thus, the effects of past treatment dose on the locomotorresponse to a subsequent cocaine challenge varied as a functionof infusion rate.

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Figure 6. The mean (±SEM) number of quadrant entries (averaged over 6 min) in response to a challenge infusion of 0.75 mg/kg cocaine over 10 sec as a function of previous cocaine dose and infusion rate (n = 6-13; see Fig. 5 legend for statistical results). When administered over 5 sec (A), all doses of cocaine tested induced a sensitized response to the challenge infusion relative to controls. When administered over 25 sec (B), none of the doses tested induced a sensitized response to the challenge relative to controls. When administered over 50 (C) or 100 (D) sec, the doses tested produced an approximately linear increase in the locomotor response to the challenge infusion, but only the 2.0 mg/kg dose differed significantly from controls. *Differs from the vehicle-pretreated (dose of 0) control group (Dunnett's tests).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It is widely accepted that the rate at which cocaine enters the brain is an important determinant of both its positive subjectiveeffects and its reinforcing effects (Gossop et al., 1992; Wingeret al., 1992; Hatsukami and Fischman, 1996), although very fewexperimental studies directly address this issue. It has beensuggested that the positive relationship between rate of drugdelivery and subjective effects may contribute to abuse liabilityand addiction (Gossop et al., 1992; de Wit et al., 1993; Hatsukamiand Fischman, 1996). However, another important effect of cocaineis its ability to induce long-lasting neuroadaptations in theorganization of brain systems that mediate its psychomotor activatingand incentive motivational effects (Robinson and Berridge, 1993,2000; Nestler and Aghajanian, 1997), and some of these neuroadaptiveprocesses have been related to the propensity for cocaine self-administrationbehavior (Piazza et al., 1989; Horger et al., 1990) and a cocaine-inducedplace preference (Lett, 1989). We hypothesized, therefore, thatthe rate of cocaine delivery may also influence its ability toinduce sensitization. To address this question, we studied onebehavioral manifestation of cocaine-induced neuroadaptations inbrain reward systems that is thought to be related to addiction:the development of psychomotor sensitization (Robinson and Berridge,1993, 2000).

In one study, rotational behavior in rats with a unilateral 6-OHDA lesion was used as an index of the psychomotor activatingeffects of cocaine (Ungerstedt and Arbuthnott, 1970; Robinson,1984). When cocaine was infused intravenously over 3-16 sec, itproduced robust behavioral sensitization. However, when infusedover 34 sec, it produced only marginal sensitization (i.e., theeffect was not statistically significant), as indicated by a challengetest given after a period of drug abstinence (modest but statisticallysignificant sensitization was observed using a within-subjectsanalysis during the drug treatment period). Similar results wereobtained in a second experiment that used locomotor activity inneurologically intact rats as an index of psychomotor activationand in which both rate of drug delivery and dose were varied.At all doses tested, cocaine induced persistent sensitization(at least 4 d) when it was administered over 5 sec. In contrast,all doses failed to induce sensitization when cocaine was administeredover 25 sec. Surprisingly, when cocaine was given over 50-100sec, its effects varied as a function of dose. At these infusionrates, there was a linear increase in the degree of sensitizationas a function of treatment dose, although significant sensitizationwas seen only at the highest dose tested (2.0 mg/kg).

It is not clear what accounts for the effect that rate of intravenous cocaine delivery has on the induction of psychomotorsensitization. One obvious explanation is that maximal brain concentrationsof cocaine may vary as a function of infusion rate, such thatthe fastest infusion rates result in higher peak brain concentrationsof cocaine than the slower infusion rates. Given that the degreeof sensitization is dose dependent (Kalivas et al., 1988; Browmanet al., 1998), the effect of infusion rate could be just secondaryto the achieved dose. There are, however, a number of reasonsto believe that this does not explain the results reported here.First, on the basis of pharmacokinetic modeling (see Materialsand Methods and Fig. 1), the peak brain concentrations of cocaineshould not differ over the range of infusion rates shown hereto influence the induction of sensitization. Second, this explanationcannot account for the fact that the fastest infusion rate (5sec) was very effective in inducing sensitization, an intermediateinfusion rate (25 sec) was ineffective, but even slower infusionrates (50-100 sec) were again effective, at least at the highestdose tested. Third, varying infusion rates between 25 and 100sec had no effect on the acute dose-locomotor effect functions.This suggests that the primary neuropharmacological effects ofcocaine (including brain concentrations of cocaine) did not varyover this range of infusion rates, although the ability of cocaineto induce sensitization varied greatly over this range of infusionrates. This is reminiscent of a report by Volkow et al. (2000)showing that in humans, smoked and intranasal cocaine producedequivalent plasma concentrations of cocaine and blockade of dopaminetransporters, but smoked cocaine produced greater self-reportsof "high." Therefore, our results are not consistent with a hypothesisthat the effect of infusion rate is simply secondary to achieveddose.

Of course, varying the intravenous infusion rate would influence the rate of cocaine entry into the brain (Fig. 1, inset).Presumably this would influence the temporal pattern of monoaminetransporter occupancy, the temporal pattern of monoamine accumulationin the synapse, and eventually, the temporal dynamics of monoaminereceptor occupancy. The implication of these results, therefore,is that the temporal dynamics of monoamine receptor occupancymay be a critical variable in initiating whatever cascade of intracellularprocesses is necessary for the persistent neurobiological adaptationsunderlying behavioral sensitization. What is especially interestingis the notion that very small changes in the temporal dynamicsof monoamine transporter occupancy (over tens of seconds) couldhave such profound effects on this form of neurobehavioral plasticity.We should stress, however, that contrary to our initial hypothesis,there does not appear to be a simple linear relationship betweenthe rate of rise of brain cocaine and susceptibility to sensitization.For example, on the basis of the pharmacokinetic model (Fig. 1),we estimated that the initial rate of rise in brain cocaine producedby 2.0 mg/kg given over 25 sec would be more than twice that producedby 0.5 mg/kg given over 5 sec, but only the latter induced sensitization.The nature of the relationship between the temporal dynamics ofcocaine delivery and sensitization remains to be determined. Nevertheless,our results are consistent with reports that the temporal patternof synaptic activation is important in producing other forms ofcellular plasticity, such as long-term potentiation (Larson etal., 1986; Greenstein et al., 1988; Tsukada et al., 1994).

The rise in extracellular dopamine produced by cocaine is tightly coupled to brain concentrations of cocaine (Nicolaysen etal., 1988). Therefore, given the pharmacokinetic model of Panet al. (1991), we would not expect that a variation in infusionrate over the range used here would influence the magnitude ofthe dopaminergic response to cocaine (although the temporal profileof the response should be affected). Indeed, it has been foundthat the peak dopamine response in the nucleus accumbens, assessedwith microdialysis, is the same when 1.0 mg/kg cocaine is givenintravenously over 6 or 150 sec (Zernig, 1997). We are not awareof any other studies that directly compare the neurobiologicaleffects of different rates of intravenous cocaine delivery, butPorrino (1993) compared the effect of intravenous versus intraperitonealcocaine on cerebral glucose utilization. She found that over awide range of doses, intraperitoneal cocaine induced glucose utilizationprimarily in structures related to nigrostriatal circuitry butfailed to change glucose utilization in components of the mesocorticolimbicsystem. In contrast, intravenous cocaine increased glucose utilizationnot only in the nigrostriatal system but also in the medial frontalcortex, nucleus accumbens, olfactory tubercle, and lateral habenula.Porrino (1993) concluded that "cocaine activates different neuronalcircuitry depending on the route by which it is administered"and that this difference was most likely the result of pharmacokinetic(i.e., rate of drug delivery) and not dose-related factors. Itis possible, therefore, that the ability of rapidly administeredcocaine to preferentially activate mesocorticolimbic circuitry(Porrino, 1993) may be related to the facilitation of psychomotorsensitization reportedhere.

Another intriguing implication of the present findings is raised by the fact that the intermediate infusion rates (e.g., 25sec) failed to induce sensitization at any dose studied and thatthe dose-effect functions for the various infusion rates wereso different. These results prompt the speculation that the neurobiologicaladaptations underlying a sensitized behavioral response in ratsgiven cocaine over 5 sec are different from those responsiblefor a sensitized behavioral response in rats given cocaine over50-100 sec. There are many different neuroadaptive processes thatcould result in an enhanced behavioral response to a drug challenge,and different neuroadaptive processes could be evoked under differentconditions. Of course, most studies of behavioral sensitizationinvolve the intraperitoneal administration of psychostimulantdrugs, which would result in relatively slow drug absorption comparedwith a 5 sec intravenous infusion (Pan et al., 1991). It is possible,therefore, that much of what is known about the neurobiology ofsensitization may not apply if sensitization is induced by modesof drug administration that result in the very rapid entry ofdrugs into the brain. This may be an important issue in thinkingabout how sensitization-related neuroadaptations contribute tothe process of addiction, because addicts tend to prefer drugs,formulations, and routes of administration that lead to the rapiduptake of drugs into thebrain.

We close with two thoughts: (1) The reason why drugs that are rapidly delivered to the brain are especially addictive maybe not because this enhances their positive subjective effects,or even their reinforcing effects, but rather because this increasestheir ability to induce sensitization-related adaptations in brainregions that mediate their incentive motivational effects (Robinsonand Berridge, 1993, 2000). (2) Drugs of abuse may produce differentcellular adaptations depending on the temporal pattern of drugdelivery. That is, although the behavioral manifestations of drugexperience-dependent changes in brain organization (psychomotorsensitization in this case) may appear similar in animals givencocaine rapidly or more slowly, the nature of the cellular adaptationsresponsible for the enhanced behavioral response may vary as afunction of the temporal pattern of drug delivery. If this istrue, it will be critical in future studies on the neurobiologyof sensitization to use procedures that capture the rapid onsetof drug effects typical in theaddict.

  FOOTNOTES

Received Oct. 12, 2001; revised Dec. 20, 2001; accepted Jan. 28, 2002.

This research was supported by Grant R01 DA02494 from the National Institute on Drug Abuse. T.E.R. was supported by a SeniorScientist Award (K05 DA00473). We are greatly indebted to Dr.J. B. Justice Jr for computing the values illustrated in Figure1.

Correspondence should be addressed to Dr. Terry E. Robinson, University of Michigan, Department of Psychology, East Hall,525 East University, Ann Arbor, MI 48109-1109. E-mail: ter{at}umich.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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