Chronic Exposure to Morphine Increases Corticosteroid-Binding Globulin

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Vol. 282, Issue 3, 1262-1268, 1997

Chronic Exposure to Morphine Increases Corticosteroid-Binding Globulin¹

Bruce Nock², Michele Wich and Theodore J. Cicero³

Washington University School of Medicine, Departments of Psychiatry and of Anatomy and Neurobiology, St. Louis, Missouri

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Although it appears that corticosterone may play an important role in determining vulnerability to drugs of abuse, few studieshave examined drug effects on factors that affect corticosteroneefficacy. Thus, studies were carried out to assess the effectsof morphine on corticosteroid-binding globulin (CBG), the majorglucocorticoid binder in blood. Since CBG-bound hormone is thoughtto be physiologically inactive, changes in CBG levels could affectcorticosterone action independently of hormone levels per se.We found that morphine caused a marked naltrexone-preventableincrease ( $approx$ 160%) in CBG in adult male rats. Elevated levels wereseen by three days and were maximal at seven days after morphinepellet (75 mg) implantation. CBG levels remained elevated whilemorphine was detectable in blood and returned toward normal asthe drug cleared from the system. A single morphine pellet wassufficient to induce a marked increase in the concentration ofCBG and two or more pellets caused maximal upregulation. Baselineand stress levels of total corticosterone (bound and unbound)were normal after chronic exposure to morphine. However, due tothe elevated level of CBG, the amount of free, physiologicallyactive hormone was dramatically reduced. These results suggestthat morphine may exert potent effects on corticosterone actionthat are not revealed by measurement of corticosterone alone.Furthermore, the increase in CBG resulting from chronic exposureto morphine might contribute to the perpetuation of drug use andto adverse effects of drug exposure by impairing normal functionsof corticosterone.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

A considerable amount of evidence from epidemiological and clinical studies now exists linking life events to drug abuse.Psychosocial stresses, in particular, appear to be associatedwith drug use (Barnet et al., 1995; Kosten et al., 1986; McFallet al., 1992) and have been hypothesized to be contributing factorsin the etiology of drug abuse (Alexander and Hadaway, 1982; Lindenberget al., 1993; O'Doherty and Davies, 1987; O'Doherty, 1991) andin relapse after remission (Krueger, 1981).

Observations from animal studies also have linked stress to drug use and, in addition, suggest the involvement of glucocorticoids.For example, repeated exposure to stressful stimuli (Deroche etal., 1995; Leyton and Stewart, 1990; Molina et al., 1994; Shahamet al., 1995) or adverse living conditions (Deroche et al., 1993a,1994) enhances psychostimulant and morphine psychomotor effectswhich may be correlated with propensity to self-administer drugs(Deminière et al., 1992; Deroche et al., 1993b; Piazza et al.,1989). This stress-induced enhancement of morphine's pharmacologicaleffects appears to be dependent upon corticosterone secretion(Deroche et al., 1993a, 1994, 1995; Piazza et al., 1994) and canbe mimicked by repeated injections of corticosterone (Derocheet al., 1992). In addition, stress or adverse living conditionspotentiate opiate (e.g., Alexander et al., 1981; Carroll et al.,1979; Dib, 1985; Shaham et al., 1993) and psychostimulant (Bozarthet al., 1989; Goeders and Guerin, 1994; Piazza et al., 1990; Ramseyand Van Ree, 1993) self-administration and reinstatement of self-administrationafter a drug free period (Shaham 1993; Shaham and Stewart, 1995).Furthermore, it appears that the propensity to self-administeris positively related to reactivity to stress and corticosteronesecretion, since rats with higher locomotor and corticosteroneresponses to novelty have a greater propensity to self-administermorphine and psychostimulants (e.g., Deroche et al., 1993b; Goedersand Guerin, 1994; Maccari et al., 1991; Piazza et al., 1991).Considering the growing amount of evidence implicating stressand corticosterone in the development of drug-seeking behaviorand in relapse after a drug-free period, it seems plausible thatglucocorticoids might also play a role in reinforcing and perpetuatingdrug use.

Thus far, surprisingly few studies have examined the effects of chronic drug exposure on glucocorticoids, and those have beenlimited almost entirely to effects on hormone levels in blood.Typically, acute exposure to morphine has been found to increaseglucocorticoid levels in many animal species, including rodents,with tolerance developing after chronic exposure (as recentlyreviewed by Pechnick, 1993). Other factors that might affect thephysiological efficacy of glucocorticoids have not been systematicallyexamined. Thus, in the studies reported here, we examined theeffects of chronic exposure to morphine on CBG (or transcortin)in adult male rats. Although CBG is known to be regulated by avariety of endogenous factors, including hormones (e.g., Galaand Westphal, 1966; Mataradze et al., 1992; Smith and Hammond,1992), there have been no previous studies of the effects of drugsof abuse on this serum protein.

CBG has a high affinity for corticosterone (K_d $approx$ 0.5 nM; see "Results" section) and is the major corticosterone-binding proteinin blood. It is generally accepted that only unbound (free) corticosteronecan gain access to target cells and initiate physiological responses(as reviewed by Mendel, 1989). CBG-bound hormone is thought tobe physiologically inactive. Thus, drug-induced changes in bloodlevels of CBG could have a significant impact on the efficacyof circulating corticosterone, which could influence ability tocope with stress and perhaps drug seeking behavior.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Animals

Male rats purchased from Harlan Sprague-Dawley, Inc. (Cumberland, IN) or bred in our colony from Harlan Sprague-Dawley stockwere used for all experiments (10-15 rats per group). The ratswere housed in groups of 2 to 3 per cage with lights in the colonyroom on from 6 A.M. to 6 P.M. They were 60 to 90 days old at thebeginning of drug treatment.

Trunk blood was collected after decapitation. All rats were sacrificed between 10 A.M. and 11 A.M. when corticosterone secretionis normally low in our colony. For sacrifice, the rats were individuallycarried by hand to a procedural room that was isolated from thecolony room. Rats were sacrificed within 15 sec of being pickedup, and no more than 60 sec elapsed between sacrifice of the firstand last rats in a cage.

Drug Treatments

Placebo, morphine (75 mg) or naltrexone (30 mg) pellets were implanted s.c. under Brevital anesthesia (40 mg/kg) and wereallowed to remain in place for the duration of the experiment.All pellets were generously provided by the National Instituteon Drug Abuse (Rockville, MD).

All naltrexone pellets were implanted on day 0. All morphine pellets also were implanted on day 0 except when specified otherwise.For the dose-response experiment, one or two morphine pelletswere implanted on day 0 or five morphine pellets were implantedsequentially. One control group received two placebo pellets onday 0. This group served as the control for the one and two morphinepellet treatments. The group receiving one morphine pellet alsoreceived one placebo pellet to equalize the number of pelletsat two for the groups. For the five pellet paradigm, morphinepellets were implanted sequentially, with one pellet implantedon day 0 and two additional pellets implanted on days 3 and 5.The control group for this treatment received the same numberof placebo pellets on the appropriate days. Since there were nosignificant differences between the two control groups, data werecombined for presentational purposes.

Stress Paradigm

When specified, rats were mildly stressed by i.p. injection of 0.7 ml physiological saline. Unstressed control rats were undisturbeduntil the time of sacrifice.

CBG Levels

CBG was measured using a protein binding assay modified from procedures described by McCormick et al. (1995). All steps werecarried out at 0°C to 4°C.

Sample preparation. Endogenous steroids were removed from serum by charcoal absorption. A 5 µl aliquot of serum was diluted to 1 ml with buffer(30 mM Tris HCl, 1 mM disodium EDTA, 10 mM sodium molybdate, 1mM dithiothreitol, 10% glycerol) containing dextran charcoal (Norit-A;5.0 mg/ml final). The mixture was vortexed, allowed to sit at4°C for 20 min and centrifuged for 15 min at 2500 rpm. Aliquotsof the supernatant fluid were diluted 1:5 with buffer and assayed.

Binding procedures. A 100 µl aliquot of steroid-free sample was incubated overnight at 4°C with 7.0 nM [³H]corticosterone with or without 16 µM corticosterone to definespecific binding (final volume = 150 µl). Ethanol (1% final) wasincluded in the incubation mixture to minimize steroid bindingto glass. Bound and free [³H]corticosterone were separated using Sephadex LH-20 columns.Columns were made from 1.0 ml plastic disposable micropipettetips stopped with a 4 mm glass bead. The column was filled withLH-20 to a height of 3.2 cm from the middle of the glass beadand equilibrated with 400 µl of buffer (30 mM Tris HCl, 1 mM disodiumEDTA, 10 mM sodium molybdate, 1 mM dithiothreitol, 10% glycerol).A 100 µl aliquot of incubation mixture was placed onto the columnand washed in with 100 µl buffer. Thirty minutes later, the samplewas eluted using 600 µl buffer. Specific binding was expressedas pmoles specific binding/ml serum or pmoles specific binding/mgserum protein, both of which gave virtually identical results.Protein content was determined by the protein-dye binding methodof Bradford (1976).

Morphine Levels in Serum

Morphine was assayed in serum using a RIA kit purchased from Diagnostic Products Corporation (Los Angeles, CA). The antibodyis highly specific for morphine with less than 0.03% cross reactivityfor morphine-3-glucuronide and less than 0.1% cross-reactivityfor morphine-6-glucuronide. The lower limit of sensitivity ofthe assay was 5 ng/ml and the standard curve was linear over therange 5 ng to 1,000 ng/ml. Intra- and interassay variability wasless than 5%.

Serum Corticosterone Levels

Unless specified otherwise, corticosterone levels refer to the total amount of corticosterone in serum. Corticosterone wasassayed in serum using a RIA kit purchased from Diagnostic ProductsCorporation (Los Angeles, CA). The antibody is highly specificfor corticosterone with less than 3% cross reactivity for 11-deoxycorticosteroneand less than 1% cross-reactivity for 18-hydroxydeoxycorticosterone,cortisol, progesterone, 17 $alpha$ -hydroxyprogesterone, dehydroepiandrosterone,aldosterone, testosterone and estradiol. The lower limit of sensitivityof the assay was 20 ng/ml, and the standard curve was linear overthe range 20 ng to 2,000 ng/ml. Intra- and interassay variabilitywere less than 5%.

CBG-bound and unbound, i.e., free, corticosterone was calculated using Pearlman's (1970; also see Plymate et al., 1987 andMcCormick et al., 1995) modification of the mass equation:

<IT>x = </IT><FENCE><IT>b − </IT><RAD><RCD><IT>b<SUP>2</SUP> − 4a/2</IT></RCD></RAD></FENCE>

where x is the molar concentration of CBG-bound corticosterone, b is the equilibrium dissociation constant for corticosteroneand CBG (K_d) plus the molar concentration of CBG (B_max) plus themolar concentration of corticosterone, and a is the molar concentrationof corticosterone times the molar concentration of CBG. Free corticosteroneis the total concentration of corticosterone minus the concentrationof CBG-bound corticosterone. K_d and B_max were determined experimentallyin the study shown in Figure 4.

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Fig. 4. Scatchard plots of [³H]corticosterone binding to CBG in vitro. Serum was pooled from rats (15/group) implanted with two placeboor morphine pellets for 7 days. B_max in serum was calculated basedon dilutions made in the binding assay (see "Materials and Methods"section). The figure shows that morphine had little or no effecton the affinity of CBG for corticosterone but increased the numberof binding sites.

Statistical Analysis

All data are expressed as mean ± standard error of the mean. t-Tests were used to compare two groups; otherwise, data weresubjected to analysis of variance followed by post-hoc analysis.Differences between groups were considered statistically significantwhen the probability that they occurred by chance was less than.05.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Figure 1 shows morphine, total corticosterone and CBG levels in serum at selected time-intervals after implantation of a singlemorphine pellet. Morphine levels were highest on Day 1 followingpellet implantation and, thereafter, declined to relatively lowlevels by Day 14. The concentration of corticosterone in serumdid not differ from control levels at any interval following morphinepellet implantation (fig. 1). CBG levels did not differ from controlvalues at one day after morphine pellet implantation. However,at three and seven days after morphine pellet implantation, CBGlevels were markedly elevated with values for the morphine exposedrats 66% (Day 3) and 97% (Day 7) higher than for controls. At14 days after pellet implantation, CBG levels in the morphineexposed group remained 20% above control values but that differencewas not statistically significant (P = .19). However, when a secondmorphine pellet was implanted on Day 7 to maintain higher morphinelevels, CBG remained significantly elevated (107%) through Day14 (fig. 1).

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Fig. 1. Serum morphine (top), total corticosterone (middle) and CBG (bottom) levels at selected time intervals after implantationof one placebo or 75-mg morphine pellet (data shown by round symbolsand solid lines). For the data shown by the square symbols anddoted lines, rats were implanted with an additional placebo ormorphine pellet on Day 7 to maintain elevated morphine levelsin blood. The figure shows that morphine had little or no effecton corticosterone but markedly increased the concentration ofCBG in serum. Implantation of a supplemental morphine pellet onDay 7 prevented the decline in CBG levels between Days 7 and 14.N = 12-13 rats/group. * indicates P < .05 vs. the placebo group.

Although only crude dose-response relationships can be established with pellets, the magnitude of morphine's effects on CBGappears to be dose-dependent. Figure 2 shows CBG levels in serumof untreated rats and of rats implanted with morphine or placebopellets. The concentration of CBG in the placebo group did notdiffer from that of untreated rats. However, as in the time-responsestudy described above, one morphine pellet caused a significantincrease in CBG. Two morphine pellets produced even higher CBGlevels, but five pellets (implanted sequentially as describedunder "Materials and Methods") caused no additional increase.None of the treatments affected the total amount of protein inserum (untreated, placebo, one, two and five pellets = 6.5 ± 0.2,6.1 ± 0.1, 6.2 ± 0.2, 6.2 ± 0.2 and 6.4 ± 0.1 ng/ml of diluted,steroid-free serum, respectively) or corticosterone levels atthe time of sacrifice (untreated, placebo, one, two and five pellets= 59 ± 16, 45 ± 11, 43 ± 12, 33 ± 10 and 40 ± 15 ng/ml, respectively).

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Fig. 2. CBG in serum of untreated adult male rats and of rats implanted with placebo or one, two or five (implanted sequentially asdescribed under "Materials and Methods"; N = 12-15 rats/group)morphine pellets 7 days earlier. The figure shows that implantationof the placebo pellets had no significant effect on CBG, whilemorphine increased CBG in a dose-dependent manner. * indicatesP < .05 vs. the placebo group.

One, two and five morphine pellets resulted in serum morphine levels of 650 ± 106, 881 ± 98 and 1515 ± 38 ng/ml, respectively,on day 7. When added directly into the in vitro assay system,morphine had little or no effect on CBG binding across that rangeof concentrations (fig. 3). Thus, the presence of morphine inthe assay system itself does not appear to affect CBG binding.

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Fig. 3. [³H]Corticosterone binding to CBG in vitro in the absence or presence of morphine. Morphine was added directly into the invitro binding assay at concentrations selected from serum morphinelevels at 7 days after implantation of one, two or five morphinepellets (see "Results" section). Serum was pooled from 12 untreatedrats. The figure shows that morphine had little or no effect onCBG binding when added directly into the assay system.

Figure 4 shows Scatchard plots of CBG binding isotherms for pooled serum taken seven days after implantation of two morphineor placebo pellets. Scatchard analysis indicated that morphinehad little or no effect on the affinity of CBG for corticosteronebut increased the number of binding sites by 140%.

In contrast to morphine, implantation of one or four naltrexone pellets had little or no effect on the concentration of CBGin serum 7, 14 or 21 days later (fig. 5). However, naltrexoneprevented the increase in serum CBG caused by morphine (fig. 6).

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Fig. 5. Serum CBG levels at selected time intervals after implantation of four placebo or one (plus placebo) or four naltrexone pellets(N = 10-13 rats/group). The figure shows that the opiate antagonisthad little or no effect on CBG at the doses and time intervalsexamined.

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Fig. 6. CBG levels at 7 days after implantation of one morphine pellet alone or in combination with four naltrexone pellets (N = 11rats/group). All pellets were implanted simultaneously. The figureshows that naltrexone blocked the morphine-induced increase inCBG. * indicates P < .05 vs. the placebo group.

Figure 7 shows total (top graph) and free (bottom graph) corticosterone in serum of unstressed or mildly stressed rats implantedwith two morphine or placebo pellets seven days earlier. The dataindicate that exposure to morphine had little or no effect onbaseline (unstressed) or stress levels of total corticosterone.However, the amount of free corticosterone, i.e., corticosteronenot bound to CBG, was markedly lower in morphine-treated ratsunder both baseline and stress conditions.

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Fig. 7. Total (top) and free (i.e., not bound to CBG; bottom) corticosterone in serum of unstressed rats (zero time-point) or ratsmildly stressed by injection of physiological saline seven daysafter implantation of two placebo or morphine pellets (N = 10-15rats/group). Free corticosterone was calculated from the meanvalues for total corticosterone using Pearlman's (1970; see "Materialsand Methods" section) modification of the mass equation and theK_d and B_max values from figure 4. The figure indicates that exposureto morphine had little or no effect on base-line (unstressed)or stress levels of total corticosterone but markedly decreasedthe amount of free corticosterone.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Chronic exposure to morphine caused a marked, time- and dose-dependent increase in the concentration of CBG in serum of adultmale rats. Elevated levels were seen by three days and appearedto be maximal at seven days after morphine pellet implantation.Thereafter, CBG levels returned toward normal as morphine clearedfrom the general circulation. Thus, morphine effects on CBG donot appear to persist significantly beyond the period when thedrug is present in the body. However, when a supplemental pelletwas implanted to maintain morphine levels, the concentration ofCBG in serum remained elevated through 14 days, the longest timeinterval examined. Morphine effects on CBG, therefore, appearto continue for as long as the drug is detectable in blood.

A single morphine pellet was sufficient to cause a marked increase in the concentration of CBG. Two pellets caused what appearedto be a maximal upregulation since no further increase was seenwith five pellets. None of the pellet implantation procedurescaused a lasting change in baseline corticosterone secretion.By the day after implantation of one morphine pellet, corticosteronelevels were normal. Corticosterone levels were also normal atseven days after implantation of two pellets and at three daysafter sequential implantation of five pellets. Thus, chronic exposureto morphine appears to affect CBG but has little effect on baselinecorticosterone levels.

The opiate antagonist naltrexone completely blocked the morphine-induced increase in CBG, indicating that morphine affectsCBG through activation of opioid receptors. We made no attemptin the current studies to identify the critical opioid receptorsubtype. In addition, our data do not establish whether the opioidreceptors are located in liver where CBG is synthesized or insome other tissue of the body. Moreover, we have little basisfor speculating about how opiate receptor activation might increaseCBG. One of the major CBG regulatory factors is corticosterone,which exerts a negative influence on CBG levels (Feldman et al.,1979; Hsu and Kuhn, 1988). Thus, a reduction in corticosteroneleads to an increase in CBG. However, acute morphine stimulatescorticosterone secretion in rats (as recently reviewed by Pechnick,1993), and chronic morphine had no apparent effect on corticosteronelevels in the present study. Therefore, the morphine-induced increasein CBG does not appear to be secondary to effects on corticosterone.

Although naltrexone blocked the morphine-induced increase in CBG, chronic exposure to the opioid antagonist alone for up to21 days did not affect CBG levels in serum. It seems likely thatthe doses tested were sufficient to antagonize the actions ofendogenous opioids, since we (Giordano et al., 1990) previouslyfound them to induce a maximal rate of opioid receptor up-regulation $---$ anindication that the activity of endogenous opioids was completelyblocked. Thus, endogenous opioids do not appear to be a significantfactor in the regulation of CBG. Whether they contribute to CBGregulation under other circumstances remains to be established.

In addition to normal baseline levels of total corticosterone, the corticosterone response to a mild stressor appeared normalat seven days after exposure to morphine. That is, morphine didnot appear to affect stress levels of total corticosterone. Thisfinding was unexpected for two reasons. First, it is at a timewhen the morphine-induced increase in CBG is maximal. Accordingly,one would expect the elevated levels of CBG to decrease the amountof physiologically active hormone and, thereby, restrict negativefeedback, causing a hyper, rather than a normal, response to stress.Jacobson et al. (1988) reported a finding that may be analogousto ours and that might shed light on this issue. They found thatthe ACTH response to i.p. injection, i.e., the stressor used inthe current study, was normal in adrenalectomized rats given corticosteronein their drinking water to mimic naturally occurring circadianchanges in corticosterone levels. Based on this and other observations,they concluded that circadian changes in corticosterone levelsmay be sufficient for normal termination of the ACTH responseto stress and that negative feedback from corticosterone mightbe unnecessary. Similarly, a restriction of negative feedbackcaused by a morphine-induced elevation in CBG appears to havelittle consequence for the magnitude and duration of the pituitary-adrenocorticalresponse to stress. Since chronic exposure to morphine has beenreported to have little or no effect on diurnal corticosteronelevels (Ignar and Kuhn, 1990; Kuki, 1979), one possibility isthat circadian variations in corticosterone are sufficient inmorphine exposed rats to maintain a normal response to stresseven in the face of elevated levels of CBG.

The second reason for not expecting to see normal stress levels of total corticosterone in morphine exposed rats is that severalprevious studies reported that chronic exposure to morphine reduced(Paroli and Melchiorri, 1961) or abolished the pituitary-adrenocorticalresponse to stress (Briggs and Munson, 1955; Buckingham and Cooper,1984). There are a number of procedural differences between thosestudies and ours that conceivably might be important. For example,in the studies by Briggs and Munson and by Buckingham and Cooperrats were anesthetized when the stress was applied. Furthermore,in all of the studies that found an inhibition of the stress response(e.g., Briggs and Munson, 1955; Buckingham and Cooper, 1984; Paroliand Melchiorri, 1961) morphine was administered at high dosesby daily injections whereas we implanted morphine pellets.

In any event, although baseline levels and the response to a mild stressor appeared normal in terms of total corticosterone,the amount of free, physiologically active hormone estimated usingPearlman's modification of the mass equation was markedly reducedunder both conditions as a result of the morphine-induced increasein CBG. This was particularly apparent at the peak of the stressresponse when the amount of free corticosterone was 90% lowerin morphine treated rats. In essence, the heightened level ofCBG dramatically blunted the response to stress. Our results thensuggest that morphine might, exert effects on endocrine physiologythrough CBG that are not apparent from hormone levels in blood.

At this point, we can only speculate about how a morphine-induced increase in CBG might contribute to drug seeking behavior.A number of possibilities seem feasible. First, in view of studiesshowing that stress can potentiate the initiation of opiate self-administration(e.g., Alexander et al., 1981; Carroll et al., 1979; Dib, 1985;Shaham et al., 1993), it seems plausible that an increase in CBGmight contribute to the perpetuation of drug use by compromisinga primary mechanism for coping with stress. Thus, a positive cascadecan be envisioned where stress potentiates the use of drugs, whichin turn compromises the individual's ability to cope with stressand, thereby, perpetuates drug use. Second, considering that corticosteroneappears to enhance psychomotor effects of opiates (Deroche etal., 1995; Leyton and Stewart, 1990; Molina et al., 1994; Shahamet al., 1995), it is conceivable that the increase in CBG andconcomitant decrease in physiologically active corticosteronewith chronic drug exposure would blunt the psychomotor effectsof morphine and, thereby, lead to a compensatory increase in druguse. Thus, an increase in CBG might contribute to the perpetuationof drug use at multiple levels.

Finally, it seems appropriate to mention that a morphine-induced increase in CBG might contribute to some adverse affectsof drug use. In particular, over the past several years, it hasbecome increasingly clear that glucocorticoids are necessary forthe development and maintenance of normal immunity (as reviewedby Jefferies, 1991). Thus, a morphine-induced increase in CBGmight impair immunity and contribute to the heightened susceptibilityof opiate addicts to infectious diseases, including HIV, and thedevelopment of AIDS (acquired immunodeficiency syndrome; Donahoeand Falek, 1988; Horsburgh et al., 1989; Lazzarin et al., 1984;Rouveix, 1992).

	Acknowledgments

We thank Michelle Gish, Jingling Chen and Edward R. Meyer for expert technical assistance.

	Footnotes

Accepted for publication May 5, 1997.

Received for publication January 27, 1997.

¹ This research was supported in part by USPHS Grants DA09344 (B.N.), DA03833 (T.J.C.) and DA09140 (T.J.C.) from the NationalInstitute on Drug Abuse.

² Recipient of Research Scientist Development Award DA00157.

³ Recipient of Research Scientist Award DA00095.

Send reprint requests to: Bruce Nock, Ph.D., Washington University School of Medicine, Department of Psychiatry, 4940 Children's Place, St. Louis, MO 63110.

	Abbreviations

ACTH, adrenocorticotropic hormone; AIDS, acquired immunodeficiency syndrome; CBG, corticosteroid-binding globulin; HIV, human immunodeficiency virus; RIA, radioimmunoassay.

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Top Abstract Introduction Materials & Methods Results Discussion References

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