Opioids Suppress IPSCs in Neurons of the Rat Medial Septum/Diagonal Band of Broca: Involvement of {micro}-Opioid Receptors and Septohippocampal GABAergic Neurons

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (26)

Citing Articles via Google Scholar

Google Scholar

Articles by Alreja, M.

Articles by Leranth, C.

Search for Related Content

PubMed

PubMed Citation

Articles by Alreja, M.

Articles by Leranth, C.

Pubmed/NCBI databases
Compound via MeSH
Substance via MeSH

Previous Article  |  Next Article

The Journal of Neuroscience, February 1, 2000, 20(3):1179-1189

Opioids Suppress IPSCs in Neurons of the Rat Medial Septum/Diagonal Band of Broca: Involvement of µ-Opioid Receptors and Septohippocampal GABAergic Neurons
Meenakshi Alreja¹^,³, Marya Shanabrough², Weimin Liu¹, and Csaba Leranth²^,³
Departments of ¹ Psychiatry, ² Obstetrics and Gynecology, and ³ Neurobiology, Yale University School of Medicine and the Ribicoff Research Facilities, Connecticut Mental Health Center, New Haven, CT 06508

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The medial septum/diagonal band region (MSDB), which provides a major cholinergic and GABAergic input to the hippocampus,expresses a high density of opioid receptors. Behaviorally, intraseptalinjections of opioids produce deficits in spatial memory, however,little is known about the electrophysiological effects of opioidson MSDB neurons. Therefore, we investigated the electrophysiologicaleffects of opioids on neurons of the MSDB using rat brain slices.In voltage-clamp recordings with patch electrodes, bath-appliedmet-enkephalin, a nonselective opioid receptor agonist, decreasedthe number of tetrodotoxin and bicuculline-sensitive inhibitorysynaptic currents in cholinergic- and GABA-type MSDB neurons.A similar effect occurred in brain slices containing only theMSDB, suggesting that opioids decrease GABA release primarilyby inhibiting spontaneously firing GABAergic neurons located withinthe MSDB. Accordingly, in extracellular recordings, opioid-sensitive,spontaneously firing neurons could be found within the MSDB. Additionally,in intracellular recordings a subpopulation of GABA-type neuronswere directly inhibited by opioids. All effects of met-enkephalinwere mimicked by a µ receptor agonist, but not by $delta$ or $kappa$ agonists.In antidromic activation studies, µ-opioids inhibited a subpopulationof septohippocampal neurons with high conduction velocity fibers,suggestive of thickly myelinated GABAergic fibers. Consistentwith the electrophysiological findings, in double-immunolabelingstudies, 20% of parvalbumin-containing septohippocampal GABA neuronscolocalized the µ receptor, which at the ultrastructural level,was found to be associated with the neuronal cell membrane. Thus,opioids, via µ receptors, inhibit a subpopulation of MSDB GABAergicneurons that not only make local connections with both cholinergicand noncholinergic-type MSDB neurons, but also project to thehippocampus.

Key words: septohippocampal; GABA; opioids; parvalbumin; septum; diagonal band of Broca

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The medial septum/diagonal band region (MSDB), which participates in learning and memory processes via its cholinergic andGABAergic projections to the hippocampus, also expresses one ofthe highest densities of opioid receptors in the brain. The opioidinnervation to the MSDB, which is comprised primarily of $beta$ endorphin-immunoreactivefibers and terminals (Watson et al., 1977; Bloom et al., 1978;Finley et al., 1981; Costa et al., 1983), originates from thehypothalamic arcuate nucleus (Millan et al., 1984). Intraseptalinjections of opioids have been reported to both increase (Botticelliand Wurtman, 1982) and decrease hippocampal acetylcholine turnover(Moroni et al., 1978) in a naltrexone-reversible manner. Behaviorally,intraseptal injections of opioids impair spatial memory, and intraseptalinjections of naltrexone enhance memory function, indicating thatopioid activity in the MSDB may normally participate in the regulationof memory processes (Bostock et al., 1988; Ragozzino et al., 1992).In addition to participating in learning and memory processes,the septal area, which is regarded as part of the reward circuit,may also contribute to the addictive properties of opioids. Ratshave been known to self-administer opioids intraseptally (Steinand Olds, 1977; Bozarth, 1983), and a marked increase in glucoseutilization (Kimes and London, 1988) and c-fos immunoreactivityoccurs in the MSDB after opioid withdrawal (Couceyro and Douglass,1995; Bot and Chahl, 1996).

The cellular targets of opioids in the MSDB that may underlie the above behavioral actions of opioids remain unknown. Thefew available studies on the electrophysiological actions of opioidsin the septal area involve extracellular recordings from unidentifiedneurons. In in vivo studies on anatomically undefined neuronsof the preoptic/septal region and the medial septal region, iontophoreticallyapplied met-enkephalin, morphine, and endorphin have been reportedto produce naloxone-reversible postsynaptic inhibitory effects(French and Siggins, 1980; Baldino and Beckman, 1982; Caretteand Poulain, 1982). Intracellular and pharmacological studieson the effects of opioids on MSDB neurons are lacking. As such,the goal of the present study was to study the physiological andpharmacological action of opioids on electrophysiologically characterizedrat MSDB neurons. Studies were performed using extracellular,intracellular, and whole-cell patch clamp recording techniquesin an in vitro rat brain slice preparation; antidromic activationstudies were used to identify septohippocampal MSDB neurons. Additionalstudies on the anatomical localization of opioid receptors onseptohippocampal neurons were performed using single- and double-immunolabelingtechniques at the light and electron-microscopiclevel.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of brain slices. Brain slices containing the MSDB were prepared from young adult male Sprague Dawley albino rats(3- to 4-weeks-old, body weight, 80-130 gm) using methods detailedpreviously (Alreja and Liu, 1996). Briefly, rats were anesthetizedwith chloral hydrate (400 mg/kg, i.p.) and killed by decapitation.To enhance the yield of healthy cells, brain slices were preparedusing artificial CSF (ACSF) in which the NaCl was initially replacedwith an equiosmolar concentration of sucrose (Alreja and Aghajanian,1995). The ACSF, pH 7.35-7.38, equilibrated with 95% O₂ and 5%CO₂, contained (in mM): NaCl, 126; KCl, 3; NaH₂PO₄, 1.25; D-glucose,10; NaHCO₃, 25; CaCl₂, 2, and MgSO₄, 2. After decapitation, thebrain was removed and placed in a Petri dish containing sucroseACSF and trimmed to yield a small block containing the MSDB. Coronalor sagittal slices of ~500 µm thickness containing the MSDB werecut with a vibrating-knife microtome (Frederick Haer) and transferredto the stage of a gas-liquid interface type of brain slice chamberover which humidified 95% O₂ and 5% CO₂ flowed. The stage temperaturewas gradually raised from room temperature to 33 ± 0.5°C over~20 min. One to 2 hr later the slice was used for recording. Thechamber was continuously perfused with normal ACSF at a rate of1-2 ml/min. Although most recordings were performed in coronalslices, sagittal slice preparations containing the dorsal fornixwere used for the antidromic activationstudies.

In most recordings from coronal slices, the slice preparation also included the lateral septum, the bed nucleus of the striaterminalis, parts of the striatum, and the ventral pallidum. However,in some coronal slice preparations, the MSDB was isolated fromall neighboring structures (including the lateral septum) by knifecuts, such that the slice contained only the MSDB (see Fig. 5B,stippled area). The purpose of these experiments was to studythe effects of opioids on MSDB neurons independent of any inputsfrom neighboring structures (seeResults).

Electrophysiological recordings were made primarily from the medial septum and from the vertical limb of the diagonal bandofBroca.

Intracellular recordings. Intracellular recordings were performed using sharp microelectrodes (25-35 M $Omega$ resistance) filledwith 2 M KCl. All recordings were made using an Axoclamp-2A (AxonInstruments, Foster City, CA) amplifier either in the bridge modeor in the discontinuous single-electrode voltage-clamp mode. Incurrent-clamp recordings, the output signal was filtered at 10kHz.

The cells selected for study had spike amplitudes of 70-100 mV. The electrophysiological criteria for identification of cholinergicand noncholinergic-type (presumably GABAergic) neurons were basedon those defined in the guinea pig and rat septum by earlier workers(Griffith and Matthews, 1986; Griffith, 1988; Markram and Segal,1990; Gorelova and Reiner, 1996). Spike durations were measuredat half-spike amplitude. In spontaneously firing cells these measurementswere done at the resting potential and in quiescent cells, firingwas evoked by injecting a small amount of depolarizing current.Input resistance was calculated by measuring the instantaneousvoltage after injection of a hyperpolarizing current. The effectsof bath-applied opioids on synaptic events were recorded onlyafter chloride loading appeared complete (~10-20min).

Discontinuous single-electrode voltage-clamp recordings were performed using previously described methods (Alreja, 1996).The cells were voltage-clamped at $-$ 60 mV. The input impedanceof each cell was continually monitored by stepping the membranepotential to $-$ 65 or $-$ 70 mV for 1 sec at 20 sec intervals. Thecurrent and voltage signals were amplified and displayed on storageoscilloscopes and also continuously recorded on a chart recorder(Gould2200).

Whole-cell recordings, acquisition, and analysis of synaptic currents. Whole-cell patch-clamp recordings were performed usingpreviously described methods (Alreja and Liu, 1996). In brief,low-resistance (2.5-3.5 M $Omega$ ) patch pipettes were filled with asolution containing (in mM): K gluconate, 120; HEPES, 10; BAPTAK₄, 5; sucrose, 20; CaCl₂, 2.38; MgCl₂, 1; K₂ATP, 1, and GTP,0.1, pH 7.32-7.35. A few experiments were done with KCl- and CsCl-containingpipette solutions. Because most recordings were performed withK gluconate-containing solutions (wherein the polarity of theIPSCs was normal and not reversed in the depolarizing direction),no attempts were made to block spontaneously occurring spikes,especially because spike characteristics were useful in the characterizationof cholinergic and noncholinergic-typeneurons.

Synaptic currents were recorded using the continuous single-electrode voltage-clamp mode. The series resistance was continuallymonitored, and cells were used for recording only if the seriesresistance was <6 M $Omega$ . Series resistance compensation was not done.If the series resistance increased during the course of the experimentand caused significant reductions in the IPSC amplitudes, effortswere made to improve access by applying one of several maneuvers(such as applying additional suction or slight positive pressure),failing which the experiment wasdiscontinued.

Spontaneously occurring IPSCs were filtered at 3 kHz, amplified 100×, and digitized at 15 kHz (to minimize distortions inthe fast rising phase of the synaptic currents) using the Digidata1200 (Axon Instruments). With gluconate-containing electrodes,IPSCs were usually acquired at a holding potential of $-$ 60 mV (unlessotherwise stated). The reversal potential of the IPSCs was estimatedby observing the amplitude and polarity of the IPSCs in each cellat different holding potentials ranging from $-$ 60 to $-$ 120 mV. WithCl-containing electrodes IPSCs were recorded at $-$ 90 mV. Ten 1 secsweeps of IPSCs were collected over 12-60 sec for each experimentalcondition. Spontaneously occurring EPSCs were blocked by bathapplication of the NMDA and non-NMDA antagonists AP-5 (50 µM)and CNQX (20 µM).

Off-line analysis of IPSCs was performed using the commercially available computer software package Axograph 2.0 (Axon Instruments),wherein the traces were visually inspected for synaptic eventsand manually marked using the mouse-measure command. This methodensured that the analysis was not corrupted by any slight changein the noise level or by membrane fluctuations. If the backgroundnoise increased during the recording, the data from that cellwas discarded. The data generated from these measurements wereused to plot cumulative probability amplitude and interevent intervalgraphs, with each distribution normalized to a maximal value of1. Cumulative probability plots obtained under different experimentalconditions were compared using the nonparametric Kolmogorov-Smirnovtest (K-S test), which estimates the probability that two cumulativedistributions differ from each other by chance alone (Van DerKloot, 1991; Lupica, 1995). The significance level for the K-Stest was set at a conservative value of p < 0.01. All numericalvalues are plotted as mean ±SEM.

Antidromic activation of septohippocampal neurons and extracellular recordings. Extracellular recordings were made from spontaneouslyfiring MSDB neurons with glass micropipettes filled with 2 M NaCl(5-10 M $Omega$ ), and the fornix was stimulated using a bipolar Teflon-coatedtungsten electrode. Septohippocampal projection neurons (SHNs)were identified by their antidromic response to electrical stimulationof the dorsal fornix (square pulses of 0.1-0.3 msec duration,40-1000 µA) using the following criteria: fixed latency of activation,high frequency following and collision of the antidromic spikeswith orthodromic spikes (see Fig. 7). Similar criteria have previouslybeen used to identify septohippocampal neurons in vivo (Lamouret al., 1984) and in vitro (Alreja and Liu, 1996; Liu and Alreja,1997; Liu et al., 1998). The threshold of activation and the latencyof antidromic activation were measured for each SHN, and the latencymeasurement was used to compute the conduction velocity for eachSHN. The distance between the stimulating and the recording electrodeswas measured using a calibrated graticule located in the eyepieceof the dissectionscope.

Reagents. All constituents of the ACSF and the patch pipette solution were obtained from Mallinckrodt and Sigma (St. Louis,MO), respectively. The tetrapotassium salt of BAPTA was obtainedfrom Molecular Probes (Eugene, OR). Bicuculline methiodide, tetrodotoxin(TTX), and Met-enkephalin were obtained from Sigma. D-Ala²,N-Me-Phe⁴,Gly-ol⁵-Enkephalin (DAMGO), [D-Pen^2,5]- Enkephalin (DPDPE), and (±)-trans-U50488 methanesulfonate (U50,488H),CTOP, 6-cyano-2,3-dihy-droxy-7-nitroquinoxaline (CNQX), and DL-2-aminophosphonovalericacid (AP-5) were obtained from Research Biochemicals (Natick,MA).

All drugs were diluted in ACSF from previously prepared stock solutions that were prepared in water (unless mentioned otherwise)and stored at $-$ 20°C. All drugs were bath-applied by turning athree-way valve that switched from ACSF to the test solution.The turnover time of the recording chamber was <30sec.

Double label fluorescent immunocytochemistry. Rats were perfused with a fixative containing 4% paraformaldehyde, 15% picricacid, and 0.1% glutaraldehyde in phosphate buffer (PB). A tissueblock containing the septum was dissected from the brain and waspost-fixed in glutaraldehyde-free fixative for 1 hr. Fifty micrometersections were cut on a Vibratome (Lancer) and washed thoroughly(four times for 10 min each) in PB between each of the followingincubation steps. First, sections were transferred into a vialcontaining 1 ml of 10% sucrose in PB. The vial was slowly immersedand frozen in liquid nitrogen and then allowed to thaw at roomtemperature. After this, the tissue was incubated for 15 min in1% sodium borohydride in PB to remove excess aldehydes. Then,the tissue was incubated overnight at room temperature in a mixtureof antibodies containing polyclonal rabbit anti-opioid µ receptor(1:500; Ab-1; Calbiochem, Cambridge, MA) plus monoclonal mouseanti-parvalbumin (1:5000; Sigma), both diluted in PB plus 0.1%sodium azide. This was followed by an incubation in the dark for2 hr at room temperature in a mixture of secondary antibodiesconsisting of goat anti-rabbit IgG-fluorescein (1:50 in PB; VectorLaboratories, Burlingame, CA) plus horse anti-mouse IgG-TexasRed (1:50 in PB; Vector Laboratories). Sections were then wetmounted onto slides, examined under an Olympus fluorescent scopeusing the appropriate filter for each fluorochrome, and the imageswerecaptured.

Mirror colocalization technique. The mirror colocalization technique of Kosaka et al. (1985) was used. Consecutive vibratomesections of the septum (20 pairs of sections per animal; a totalof three animals) were placed in alternate wells of a 24-welltissue culture plate. Every other section was immunostained forparvalbumin (PA) while each corresponding serial section was immunolabeledfor µ-opioid receptor. In this experiment, a polyclonal rabbitanti-PA (1:3000; a gift of Dr. Kenneth G. Baimbridge, Universityof British Columbia, Vancouver, British Columbia, Canada) anda rabbit anti-µ-opioid receptor antibody (1:2500; Calbiochem)were used. Each antiserum was diluted in 1% normal goat serumin PB containing 0.1% sodium azide. Sections were incubated inthe primary antisera overnight at room temperature. This was followedby incubation in the secondary antiserum, biotinylated anti-rabbitIgG (1:250 in PB; Vector Laboratories), and then, in avidin-biotin-peroxidase(ABC Elite, 1:50 in PB; Vector Laboratories), each for 2 hr atroom temperature. The tissue-bound peroxidase was visualized witha diaminobenzidine (DAB) reaction (15 mg DAB, 165 µl of 0.3% H₂O₂in 30 ml PB). The sections were washed (four times for 10 mineach) between each incubation step. Consecutive sections weremounted on slides (two sections per slide; one immunostained forPA and the other for µ-opioid receptor) in such a way that theposterior side of the first section and the anterior side of thesecond section were face up. Slides were dehydrated and coverslippedin Permount. Light-microscopic examination and photographs weretaken from consecutive sections of the same identified perikaryato determine colocalization of the twosubstances.

Immunostaining for electron microscopy. Sections for electron microscopy were first incubated in a 1% sodium borohydride inPB solution. After thorough washing, the sections were freeze-thaw-treated(see above). Immunostaining for µ-opioid receptor was performedusing the same protocol as for the mirror colocalization technique.After the DAB reaction, sections were postosmicated (1% OsO4 inPB for 15 min), dehydrated through increasing concentrations ofethanol (the 70% ethanol contained 1% uranyl acetate, 30 min),and then embedded in Araldite. Ultrathin sections were cut ona Reichert-Jung ultramicrotome, placed on Formvar-coated single-slotgrids, and examined under a Philips CM-10 electronmicroscope.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Met-enkephalin suppresses inhibitory synaptic activity in both cholinergic and noncholinergic-type MSDB neurons

In intracellular recordings performed with sharp microelectrodes containing KCl, both cholinergic-type and noncholinergictype neurons were observed in the MSDB (Fig. 1). Bath-applicationof the nonselective opioid agonist, met-enkephalin (10-100 µM;in absence of peptidase inhibitors) decreased the number of spontaneouslyoccurring depolarizing synaptic potentials in both types of MSDBneurons. This effect was blocked by the nonselective opioid antagonistnaloxone (n = 3; Fig. 1). In whole-cell recordings with K gluconate-containingelectrodes, the effect of bath-applied met-enkephalin was seenas a decrease in the number of hyperpolarizing synaptic potentials.These observations suggested that the depolarizing synaptic potentialsrecorded with Cl-containing electrodes may in fact be reverse IPSPs (see below).

View larger version (10K):
[in this window]
[in a new window]
Figure 1. Bath applications of met-enkephalin, a nonselective opioid agonist, decreases synaptic activity in both cholinergic and noncholinergic-type MSDB neurons. A, B, Intracellular recordings with KCl-containing electrodes show cholinergic and noncholinergic-type MSDB neurons. A, A spontaneously firing broad-spiked cholinergic-type MSDB neuron (spike duration, 0.8 msec). Note the prominent slow afterhyperpolarization, which is characteristic of septal cholinergic neurons. Note that bath-applied met-enkephalin (100 µM) decreased depolarizing synaptic potentials in this neuron. B, Met-enkephalin also decreased the number of depolarizing synaptic potentials in a quiescent, sharp-spiked, noncholinergic-type (presumably GABAergic) MSDB neuron (spike duration, 0.3 msec). Note the prominent fast afterhyperpolarization and the depolarizing sag (in response to the hyperpolarizing pulse) that are characteristic of MSDB GABAergic neurons. C, The nonselective opioid antagonist naloxone blocked the inhibitory effect of enkephalin on spontaneously occurring synaptic potentials.

To further analyze the effect of met-enkephalin on synaptic activity in MSDB neurons, recordings were performed in the voltage-clampmode using low-resistance whole-cell electrodes containing K gluconateor CsCl. Spontaneously occurring IPSCs were observed in 58.2%of the neurons tested (39 of 67); met-enkephalin inhibited thespontaneously occurring IPSCs in 56.4% (22 of 39) of the cellstested (Fig. 2). The amplitude and polarity of the opioid-sensitiveIPSCs varied with changes in E_Cl-. Thus, with gluconate-containingelectrodes (calculated E_Cl- = $-$ 80 mV), the amplitude of the spontaneoussynaptic currents decreased at more negative holding potentialsand reversed polarity between $-$ 80 and $-$ 100 mV in all cells tested.The actual reversal potential was $-$ 88 ± 6 mV (Fig. 2). In recordingswith chloride-containing electrodes (calculated E_Cl- = 1.5 mV),the opioid-sensitive synaptic activity was reversed in polarity(see Figs. 1, 4, 5), and the amplitude of the synaptic eventsincreased at more negative holding potentials.

View larger version (34K):
[in this window]
[in a new window]
Figure 2. Met-enkephalin-sensitive synaptic activity reverses polarity near the chloride equilibrium potential and is blocked by the GABA_A receptor antagonist bicuculline. A, Whole-cell current-clamp recording from a GABA-type MSDB neuron with a K-gluconate-containing patch electrode. Note the fast afterhyperpolarization and the depolarizing sag. Consecutive 0.5 sec traces show spontaneously occurring IPSCs recorded under different experimental conditions. The first sets of traces show IPSCs recorded at $-$ 60 mV under control conditions, with met-enkephalin and after washout of met-enkephalin. Subsequent sets of traces show IPSCs recorded under control conditions at different holding potentials (ranging from $-$ 60 to $-$ 120 mV). Note the changes in amplitude and polarity of the synaptic currents at different holding potentials. The bar chart summarizes the data shown above. The mean IPSC amplitude under control conditions is plotted against different holding potentials. Note that the mean amplitude of the met-enkephalin-sensitive IPSCs decreased at more negative holding potentials and reversed polarity between $-$ 80 and $-$ 90 mV, which is close to the calculated E_Cl- of $-$ 80 mV. This experiment was done in presence of 20 µM CNQX and 50 µM AP-5 to block excitatory synaptic currents. B, In this cell, bicuculline blocked the spontaneously occurring IPSCs in a reversible manner. Subsequent sets of traces show the inhibitory effect of met-enkephalin. Note that the µ-selective opioid receptor agonist DAMGO mimicked the effect of met-enkephalin. All drugs were applied consecutively to the same cell.

As mentioned above, neurons that exhibited enkephalin-sensitive synaptic activity did not have similar electrophysiologicalcharacteristics but belonged to two classes of electrophysiologicallydistinct subgroups (Fig. 1). Of a total of 67 neurons tested usingwhole-cell electrodes, 24 neurons were electrophysiologicallyidentified as cholinergic-type, and the remaining 43 as noncholinergic(presumably GABAergic). This characterization was based on criteriapreviously defined by other investigators (Griffith and Matthews,1986; Griffith, 1988; Markram and Segal, 1990; Gorelova and Reiner,1996). Cells classified as cholinergic-type (Fig. 1A) had broadspikes (0.7-1.3 msec) and prominent slow afterhyperpolarizations(AHPs) showed classical rectification but lacked a prominent depolarizingsag in the electronic response to a hyperpolarizing pulse (Fig.1C). Spontaneously occurring inhibitory synaptic activity waspresent in 11 of 24 cholinergic-type neurons tested; enkephalinsuppressed this activity in 4 of 11 neurons tested; an opioid-inducedoutward current was observed in 2 of 24 neuronstested.

The remaining 43 cells, classified as noncholinergic-type (Figs. 1B, 2, 8A) had shorter duration spikes (0.25-0.5 msec), prominentfast AHPs, and most displayed depolarizing sags on hyperpolarization.Enkephalin suppressed spontaneously occurring synaptic activityin 20 of 43 neurons tested, and an opioid-induced outward currentwas observed in 25% of the neuronstested.

Met-enkephalin suppressed IPSCs are GABAergic in nature and result from a firing of GABAergic neurons within the MSDB

Because the above-mentioned data suggested that the opioid-sensitive synaptic currents are inhibitory in nature, we hypothesizedthat the spontaneously occurring IPSCs that are observed in cholinergicand noncholinergic-type MSDB neurons may be originating from GABAergicneurons within the septal nuclei. Therefore, we tested the effectof bicuculline, a GABA_A antagonist, and tetrodotoxin, a fast sodiumchannel blocker, on the opioid-sensitive Cl-mediated synaptic activity. Both bicuculline (Fig. 2B; n = 3)and tetrodotoxin, a fast sodium channel blocker (Fig. 4; n = 4),blocked the spontaneously occurring inhibitory synaptic activity,suggesting that a major effect of opioids in the MSDB is to inhibitIPSCs that are both trans-synaptic and GABAergic in nature. Acomparison of the frequency and amplitude distribution of thesIPSCs was performed before and after bath application of met-enkephalinusing patch electrodes containing CsCl (n = 7). Met-enkephalinsignificantly altered both the frequency and the amplitude distributionof the sIPSCs, as assessed by the K-S test (Figs. 3, 4). The changein the frequency and amplitude distributions of the sIPSCs presumablyoccurs because of an opioid-induced loss of action potential-dependentIPSCs after hyperpolarization of GABAergic neurons (Cohen et al.,1992; Lupica, 1995).

View larger version (28K):
[in this window]
[in a new window]
Figure 3. Opioids alter both the frequency and amplitude distribution of sIPSCs. A, Whole-cell voltage-clamp recording from an MSDB neuron with a CsCl-containing patch electrode. EPSCs were blocked using glutamate receptor antagonists (see Materials and Methods). Consecutive 0.5 sec traces show spontaneously occurring IPSCs recorded at $-$ 90 mV before and after bath application of met-enkephalin. Note the reversed polarity of the IPSCs. B, C, Cumulative amplitude and frequency distributions of sIPSCs constructed from data shown in A. Note that both the amplitude and frequency distribution were statistically different under the two experimental conditions (p < 0.0001 for amplitude distribution and p < 0.005 for frequency distribution, 274 events analyzed for control and 222 events for met-enkephalin). This presumably reflects loss of action potential-dependent IPSCs after hyperpolarization of GABAergic neurons. D, Bar chart summarizes the effect of met-enkephalin and the µ agonist DAMGO on the frequency of sIPSCs recorded with K gluconate or CsCl-containing patch electrodes. Both met-enkephalin and DAMGO produced a significant decrease in the frequency of sIPSCs (p < 0.001, Student's t test).

View larger version (23K):
[in this window]
[in a new window]
Figure 4. TTX blocks spontaneously occurring IPSCs in MSDB neurons. A, Whole-cell voltage-clamp recording from an MSDB neuron with a CsCl-containing patch electrode. EPSCs were blocked using glutamate receptor antagonists (see Materials and Methods). Consecutive 0.5 sec traces show spontaneously occurring IPSCs recorded at $-$ 90 mV before and after bath application of DAMGO and in presence of TTX. Note that DAMGO blocked spontaneously occurring IPSCs and that a subsequent application of TTX blocked the IPSCs. B, C, Cumulative amplitude and frequency distributions of sIPSCs constructed from data shown in A. Note that both the amplitude and frequency distribution were statistically different in the presence of DAMGO (p < 0.0001 for amplitude distribution and p < 0.005 for frequency distribution as compared to control). This presumably reflects loss of action potential-dependent IPSCs after hyperpolarization of GABAergic neurons. The distributions recorded under control and washout conditions were not statistically different from each other.

To determine if opioids have an additional effect on the TTX-insensitive spontaneous release of GABA from nerve terminals,we tested the effects of opioids and TTX on spontaneously occurringinhibitory synaptic currents recorded with patch electrodes containingCsCl. CsCl, by improving the integrity of the voltage clamp, enhancesthe detectability of miniature IPSCs (mIPSCs). As expected, opioid-sensitiveIPSCs were blocked by TTX, however, despite the markedly improvedsignal-to-noise ratio with CsCl electrodes (noise level, 5-10pA), TTX-insensitive mIPSCs were essentially undetectable in MSDBneurons in the four cells tested (Fig. 4), rendering it unfeasibleto test the effect of opioids on mIPSCs in MSDB neurons. Thus,although the present study cannot rule out an effect of opioidson miniature IPSCs in MSDB neurons; it provides strong evidencethat the primary effect of opioids in MSDB neurons is to inhibitimpulse-dependent GABA release that is caused by firing of GABAergicneurons. We have adopted the term "spontaneous" to describe theseTTX-sensitive events; thus, the term spontaneous IPSCs (sIPSCs)simply means the synaptic currents have not been evoked via exogenouselectrical stimulation and that sIPSCs are evoked by the actionpotential discharge of neurons and serve as an index of firingrate and hence excitability state of aneuron.

Theoretically, the opioid-sensitive inhibitory synaptic activity, that is TTX-sensitive, could originate from a firing ofGABAergic neurons present within the MSDB or from GABA neuronspresent in other brain structures located within the slice preparation(Fig. 5A). Of the brain regions present in our slice preparation(Fig. 5A, stippled area), the lateral septum was of special interestbecause not only does it contain a large population of GABA neuronsbut also expresses opioid receptors; until recently the lateralseptum was believed to provide a massive GABAergic input to theMSDB (Leranth et al., 1992). To determine whether the TTX-sensitiveIPSCs that are inhibited by opioids originate from GABA neuronswithin the MSDB, we tested the effects of met-enkephalin in brainslices where the MSDB had been surgically isolated from all neighboringstructures such as the lateral septum (Fig. 5B, stippled area).The opioids induced a similar decrease in synaptic activity inboth types of slice preparations. Similar to the control slicepreparation, in the isolated MSDB slice preparation, spontaneouslyoccurring IPSCs were present in 54.5% of the neurons tested (6of 11); met-enkephalin inhibited the spontaneously occurring IPSCsin four of six cells that showed spontaneously occurring IPSCs.Thus, the opioid-sensitive synaptic activity that is observedin cholinergic and GABA-type MSDB neurons originates from GABAneurons and terminals present within the MSDB. Because most ofthe opioid-sensitive synaptic activity in MSDB neurons is blockedby TTX, our results suggest that TTX-sensitive IPSCs that aresuppressed by opioids originate from GABA neurons present withinthe MSDB.

View larger version (26K):
[in this window]
[in a new window]
Figure 5. Opioid-sensitive IPSCs originate from within the MSDB. A, Consecutive 1 sec traces show spontaneously occurring IPSCs recorded at a holding potential of $-$ 60 mV under different experimental conditions. This whole-cell recording was made in a slice preparation that contained the MSDB as well as other neighboring brain structures (stippled area), such as the lateral septum (ls). Note that met-enkephalin decreased the number of sIPSCs. Also note that this effect was mimicked by the selective µ-opioid receptor agonist DAMGO, suggesting involvement of µ-opioid receptors. B, This whole-cell recording was made from a brain slice that contained only the MSDB (stippled area). Note that the spontaneously occurring IPSCs were inhibited both by met-enkephalin and DAMGO. Because the slice preparation contained only the MSDB, it can be concluded that met-enkephalin and DAMGO suppress sIPSCs that originate from within the MSDB. The amplitude and frequency distributions were statistically different under control and test conditions.

The µ-opioid receptor mediates the suppressive effect of opioids on IPSCs in MSDB neurons

Receptor mRNA (Mansour et al., 1994; Delfs et al., 1994; Zastawny et al., 1994) and autoradiographic studies (Goodman andPasternak, 1985; Mansour et al., 1988) have revealed high levelsof both µ- and $delta$ -opioid receptor message in neurons of the MSDB.To determine the receptor subtype or subtypes mediating the effectsof opioids on IPSCs, we tested the effect of DAMGO, a µ-selectiveagonist, and DPDPE, a $delta$ -selective agonist, on met-enkephalin-sensitiveIPSCs (Figs. 2, 3D, 4, 5). DAMGO mimicked the effect of met-enkephalinand suppressed sIPSCs in all seven cells tested; DPDPE had littleor no effect in any of the three cells tested. Note that DAMGOalso mimicked the effect of enkephalin in slices that containedonly the MSDB (Fig. 5B). To further confirm the involvement ofthe µ-opioid receptor, we tested the effect of the µ-selectiveantagonist CTOP. CTOP blocked the effect of met-enkephalin andDAMGO in the three cells tested (data notshown).

Opioid-induced inhibition of septohippocampal GABA-type neurons

Based on the above observations, we hypothesized the existence in the MSDB of a subpopulation of spontaneously firing GABAergicneurons that would be directly inhibited by opioids. As a firststep, we looked for spontaneously firing neurons in the MSDB usingthe extracellular recording technique and tested the effect ofopioid peptides on these spontaneously firing neurons. Consistentwith our hypothesis, we found a subpopulation of spontaneouslyfiring neurons that were inhibited by met-enkephalin (57% of thespontaneously firing cells tested; 25 of 44). The µ-selectiveagonist DAMGO mimicked the effect of met-enkephalin in all sevencells tested; DPDPE had little effect in the two cells tested(Fig. 6A).

View larger version (32K):
[in this window]
[in a new window]
Figure 6. Opioids inhibit a subpopulation of spontaneously firing MSDB neurons. A, B, Extracellular recording from a spontaneously firing MSDB neuron showing the inhibitory effect of met-enkephalin. Note that the µ agonist DAMGO mimicked the inhibitory effect of met-enkephalin in a concentration-dependent manner and that DPDPE had very little effect. C, Summarizes the effect of met-enkephalin (100 µM) and DAMGO (100 nM) on spontaneously firing MSDB neurons. The smaller effect of DAMGO as compared to met-enkephalin was caused by the submaximal concentration used (A). An inhibitory effect of opioids was observed in 57% of spontaneously firing MSDB neurons tested.

Because a subpopulation of MSDB GABAergic neurons project to the hippocampus, we next asked the question $---$ do the spontaneouslyfiring neurons that are inhibited by met-enkephalin project tothe hippocampus? To answer this question, we tested the effectof met-enkephalin on 25 antidromically activated, spontaneouslyfiring septohippocampal neurons recorded in sagittal brain slicepreparation (Fig. 7A). Interestingly, 76% of the neurons tested(19 of 25) responded to met-enkephalin with a decrease in firingrate, and DAMGO mimicked the effect of enkephalin in all threecells tested (Fig. 7B-D). More importantly, all the neurons sensitiveto met-enkephalin had fast conducting fibers with a mean conductionvelocity of 1.83 ± 0.14 m/sec (range, 1.1-3.2 m/sec). Conductionvelocities in this range are highly suggestive of GABAergic neurons(see Discussion). Figure 7D is a summary of the abovementionedextracellular data on septohippocampal neurons.

View larger version (38K):
[in this window]
[in a new window]
Figure 7. Opioids inhibit a subpopulation of spontaneously firing, antidromically activated septohippocampal neurons. A, Sagittal section through the rat brain, showing the septal area. The boxed area is enlarged (right) and shows the MSDB, which was the recording site. For antidromic activation of septohippocampal neurons, the stimulating electrode was placed in the dorsal fornix because it conveys both cholinergic and GABAergic MSDB fibers to the hippocampus. B, Extracellular recording from a spontaneously firing antidromically activated septohippocampal neuron. A spontaneous spike was used to trigger the oscilloscope (TS), the dorsal fornix was stimulated (*) 3 msec later, and an antidromically activated spike (AS) was obtained after a latency of 0.7 msec (left trace). This cell was classified as GABA-type based on the calculated conduction velocity of 2.2 m/sec. The right trace shows a positive collision test, wherein the cell could not be activated antidromically when the dorsal fornix was stimulated 0.3 msec after the triggering spike (approximately half the antidromic latency). This and other cells were also confirmed to be antidromically activating using additional criteria (see Materials and Methods). Stimulation current, 75 µA, 0.3 msec. C, Chart record showing the effect of met-enkephalin on the firing rate of a spontaneously firing septohippocampal neuron (same cell as shown in B, above). D, Summarizes the effect of a near-maximal concentration of met-enkephalin (100 µM) and a submaximal concentration of DAMGO (100 nM) on antidromically activated SHNs. The smaller effect of DAMGO as compared to met-enkephalin was attributable to the submaximal concentration used (Fig. 6). An inhibitory effect of opioids was observed in 76% of spontaneously firing SHNs tested.

In addition to having fast-conducting fibers, noncholinergic (presumably GABAergic) neurons have been reported to exhibitelectrophysiological properties distinct from cholinergic-typeneurons. We therefore made use of both the whole-cell and thesharp microelectrode intracellular recording technique to lookfor GABA-type neurons in the MSDB and tested the effect of opioidson their membrane properties. The GABA-type neurons tested hadshort-duration spikes (0.4 ± 0.02 msec), a prominent fast butnot a slow AHP, and a low input resistance (<125 M $Omega$ ). Some ofthe cells also exhibited a prominent depolarizing sag in responseto hyperpolarizing pulses. Using whole-cell recordings with Kgluconate-containing patch electrodes, we tested the effect ofMet-enkephalin on 37 GABA-type neurons. Met-enkephalin had noeffect in 37.8% (14 of 37) of the GABA-type neurons tested, andit reduced ongoing inhibitory synaptic activity by 59 ± 5.8% in45.9% of the cells tested (17 of 37). In 24.3% of the cells tested(9 of 37), met-enkephalin produced either a small hyperpolarization(under current-clamp conditions) or a small outward current (undervoltage-clamp at $-$ 60 mV). In intracellular electrodes with KCl-containingsharp microelectrodes, met-enkephalin produced a similar membraneresponse in 8 of 27 cells tested (29.6%). Thus, the percentageof GABA-type cells that responded to met-enkephalin did not varywith the type of recording used. The opioid-responsive GABA-typecells had a mean spike duration of 0.35 ± 0.01 msec and an inputresistance of 91 ± 15 M $Omega$ (n = 17); 12 of 17 cells were spontaneouslyfiring; 14 of 17 cells displayed a prominent depolarizing sagin response to a hyperpolarizing pulse. The data from both theserecordings is therefore summarizedtogether.

Under voltage-clamp conditions at $-$ 60 mV met-enkephalin produced a small change in the holding current (range, 20-120 pA;mean, 45 ± 11.4 pA; n = 9). This current was associated with anincrease in input conductance (Fig. 8B), suggesting a net openingof channels. Current-voltage curves performed using slow steady-stateramps ( $-$ 60 to $-$ 120 mV in 10 sec) before and during opioid treatmentrevealed an increase in inward rectification and an outward currentthat reversed polarity close to the potassium equilibrium potential(data not shown). Under current-clamp conditions, the effect ofmet-enkephalin was observed as a 1-12 mV hyperpolarization (mean,4.7 ± 1.4 mV; n = 9; Fig. 8A). In the three cells tested, theopioid-induced outward current persisted in the presence of TTX,suggesting the presence of a direct postsynaptic effect. DAMGOmimicked the effect of enkephalin and produced an outward currentin the three cells tested; the effect of met-enkephalin was alsoblocked by the µ antagonist CTOP. DPDPE (n = 3) and U50,488H (n= 2) had very little or no effect in the cells tested (Fig. 8B).Because only a small percentage of GABA-type neurons respondedto opioids with a direct effect and that too with a small current,we were unable to perform concentration-response curves with theagonists.

View larger version (34K):
[in this window]
[in a new window]
Figure 8. Opioids inhibit a subpopulation of GABA-type MSDB neurons and induce a direct, µ receptor-mediated outward current. A1, A2, Whole-cell current-clamp recording from a GABA-type MSDB (spike duration, 0.29 msec). Also note the pronounced depolarizing sag in response to the hyperpolarizing pulses (0.5 nA steps). A3 shows the resting membrane potential recorded from the same cell. Note that the met-enkephalin effect reversed on washout. B1 and B2 show effect of different opioid receptor agonists in another GABA-type neuron that was voltage-clamped at $-$ 60 mV (characteristics not shown). Met-enkephalin produced a 50 pA outward current. This effect was mimicked by the µ-opioid receptor agonist DAMGO, but not by the $delta$ -receptor agonist DPDPE. The $kappa$ receptor agonist U50488H also had no effect on this cell (data not shown). Pretreatment with the µ receptor antagonist CTOP blocked the inhibitory effects of met-enkephalin and DAMGO. Input conductance was measured by stepping the membrane potential to $-$ 70 mV for 1 sec every 20 sec. Note that both met-enkephalin and DAMGO increased the input conductance of the cell. The taller intermittent deflections indicate the time at which the cell membrane was stepped to $-$ 120 mV. In this cell, the opioid-induced outward current reversed near E_K ( $-$ 92 mV; data not shown). Both the outward current and the accompanying conductance change were blocked by the opioid antagonist CTOP. An inhibitory effect of opioids was observed in 24.3% of GABA-type neurons tested; this effect persisted in the presence of TTX in the three cells tested.

Thus, consistent with our hypothesis, GABA-type neurons that respond to µ-opioid receptor agonists were found within theMSDB.

To corroborate the above electrophysiological findings, we performed immunostaining for the µ-opioid receptor in MSDB neuronsand also combined it with immunolabeling for parvalbumin, a Ca²⁺-binding protein that is expressed only by septohippocampal GABAneurons in the MSDB (Freund, 1989) and hence has been used asa marker for septohippocampal GABAneurons.

Immunostaining for µ-opioid receptor in MSDB neurons

Immunostaining for the µ-opioid receptor resulted in a large number of immunopositive cells in the septum. In the lateralseptum, the majority of these profiles could be observed in thedorsolateral area of this septal region. In contrast, in the MSDBcomplex, µ-opioid receptor-containing cells were homogeneouslydistributed. Immunoreactivity was associated mostly with somataand large processes (Fig. 9a), however, immunoreactive punctacould also be observed. Electron microscopic analysis performedexclusively on MSDB µ-opioid receptor-immunoreactive cells revealedthat all of these cells are neurons. The major characteristicof these neurons was that they contained infolded nuclei (Fig.9b). Glial elements were always immunonegative. In the somataof these immunopositive neurons, the immunoreaction was mostlyassociated with the inner surface of the cell membrane.

View larger version (202K):
[in this window]
[in a new window]
Figure 9. Light (a) and electron (b) micrographs demonstrate the result of immunostaining for µ-opioid receptor in the medial septum. Immunoreactivity for µ-opioid receptor is present in somata and large processes (arrowheads). The electron micrograph shows a µ-opioid receptor-immunoreactive neuron (N) characterized by an infolded nucleus. A neighboring glia cell (G) is free of reaction product. Note that in the immunostained neuron, the reaction product is mostly associated with the inner cell membrane. Scale bars: a, 20 µm; b, 1 µm.

Colocalization of µ-opioid receptor and parvalbumin in MSDB neurons

The colocalization studies were performed exclusively in the MSDB using two different types of experiments, double immunofluorescenceand the "mirror" colocalization technique. First, a double immunofluorescenceexperiment was performed. The results of this colocalization seemedto indicate that a significant percentage of the µ-opioid receptor-immunoreactiveneurons of the medial septum co-contain parvalbumin, a calcium-bindingprotein (Fig. 10).

View larger version (53K):
[in this window]
[in a new window]
Figure 10. Colocalization of µ-opioid receptor with parvalbumin-containing MSDB neurons using the technique of double immunofluorescence. Two pairs of color light micrographs (a and b; c and d) demonstrate three neurons (arrowheads) immunoreactive for both parvalbumin (immunolabeled with Texas Red; a and c) and µ-opioid receptor (immunostained with FITC; b and d) in the medial septum. Asterisks label the same capillaries. Scale bar, 20 µm.

However, because the double immunofluorescence technique can lead to errors in interpretation because of the possibility ofan overlap in the emission spectra of the fluorochromes, uncontrollablecross-reactivity between immunoreagents, and because of the quicknesswith which the fluorochromes fade under light microscopic examination(which makes an in-depth analysis very difficult), the mirrorcolocalization technique was also used. The mirror colocalizationtechnique has the advantage of being absolutely specific becauseimmunostaining for the two tissue antigens is performed on separatesections. Sections from three animals (60 pairs of sections) wereexamined. This analysis revealed that ~50% of the µ-opioid receptor-immunopositiveneurons demonstrated immunoreactivity for PA. Only ~20% of thePA-immunopositive neurons of this area co-contained µ-opioid receptors(Fig. 11).

View larger version (79K):
[in this window]
[in a new window]
Figure 11. Colocalization of µ-opioid receptor with parvalbumin-containing MSDB neurons using mirror colocalization technique. Light micrographs show the result of a mirror colocalization experiment for parvalbumin (a) and µ-opioid receptor (b) on a pair of consecutive vibratome sections of the medial septal area. A large population (numbered arrows) of parvalbumin-immunoreactive neurons exhibits immunoreactivity for µ-opioid receptor. Asterisks label identical capillaries. Scale bar, 20 µm.

Thus, consistent with electrophysiological findings a small subpopulation of septohippocampal GABAergic neurons were foundto express the µ-opioidreceptor.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The main finding of this study is that opioids suppress inhibitory synaptic activity in both cholinergic and GABA-type medialseptal/diagonal band neurons; this decrease in inhibitory activityresults primarily from a direct µ receptor-mediated inhibitionof a small subpopulation of GABA-type neurons that not only makenumerous local connections but also project to the hippocampus.Thus, opioid effects in the MSDB are likely to have a profoundeffect on septal as well as septohippocampalfunctions.

Opioids inhibit GABAergic neurons in the MSDB brain slice preparation

In the present study, bath-applied met-enkephalin, a nonselective opioid agonist, decreased the frequency of spontaneouslyoccurring inhibitory synaptic activity in both cholinergic andnoncholinergic-type (presumably, GABAergic) MSDB neurons. Thespontaneously occurring inhibitory synaptic potentials were blockedby bicuculline, a GABA_A receptor antagonist. The change in theamplitude and polarity of the inhibitory synaptic currents wasalso consistent with changes in the E_Cl-. Thus, in recordingswith gluconate-containing electrodes (calculated E_Cl- = $-$ 80 mV),the amplitude of the spontaneously occurring synaptic currentsdecreased at more negative holding potentials and reversed polaritybetween $-$ 80 and $-$ 100 mV, whereas with chloride-containing electrodes(calculated E_Cl- = 1.5 mV), the IPSCs were reversed in polarityand showed an increase in amplitude at more negative holding potentials.Additionally, opioid-sensitive IPSCs were blocked by tetrodotoxin(a fast sodium channel blocker), suggesting that in the MSDB opioidsinhibit impulse-dependent GABArelease.

The present study, however, does not rule out an additional effect of opioids on miniature IPSCs in MSDB neurons. As mentionedin the results, TTX-insensitive mIPSCs, representing terminalGABA release, were barely detectable under our low-noise (5-10pA) experimental conditions in MSDB neurons. This is interestingas in the CA1 hippocampal pyramidal cells, opioid-sensitive mIPSCs,which occur at frequencies of 2-20 Hz and are 5-100 pA in amplitude(which is above the noise level in our recordings), can be readilydetected with CsCl or even with KCl-containing electrodes (Cohenet al., 1992; Lupica, 1995). The reason for this difference betweenthe MSDB and the hippocampus remains unclear. Thus, the primaryeffect of opioids in MSDB neurons is to inhibit impulse-dependentGABA release that is caused by firing of GABAergicneurons.

It was also concluded that the opioid-induced changes in inhibitory synaptic activity result primarily from an inhibitionof GABAergic neurons located within the MSDB because (1) opioidsinduced a similar decrease in IPSCs in slices in which the MSDBhad been surgically isolated from all neighboring brain structuressuch as the lateral septum, confirming that opioid-inhibited IPSCsoriginate from within the MSDB; (2) spontaneously firing MSDBneurons that were inhibited by opioid agonists were found withinthe MSDB complex; and (3) in voltage-clamp recordings, GABA-typeneurons that were directly inhibited by met-enkephalin in a tetrodotoxin-insensitivemanner were also found within the MSDBcomplex.

The µ-opioid receptor mediates the effect of met-enkephalin on MSDB GABAergic neurons

It was concluded that the µ-opioid receptor mediates the effect of met-enkephalin on MSDB GABAergic neurons because the µbut not the $delta$ or $kappa$ receptor agonists mimicked the observed effectsof met-enkephalin and decreased the frequency of bicuculline andTTX-sensitive spontaneously occurring IPSCs both in preparationscontaining the MSDB and neighboring brain structures as well asin preparations containing only the MSDB. Similarly, the µ agonistalso mimicked the effect of met-enkephalin and blocked the activityof spontaneously firing MSDB neurons recorded extracellularly,it also mimicked the direct effect of met-enkephalin in GABA-typeneurons and produced a TTX-insensitive outward current. Thesefindings are consistent both with the high levels of µ receptorbinding (Goodman and Pasternak, 1985; Mansour et al., 1988) andreceptor mRNA (Delfs et al., 1994; Mansour et al., 1994; Zastawnyet al., 1994) in the MSDB. A similar opioid receptor-mediateddecrease in sIPSCs as a result of inhibition of GABAergic neuronshas been reported in other areas of the brain such as the hippocampus(Zieglgansberger et al., 1979; Nicoll et al., 1980; Siggins andZieglgansberger, 1981; Cohen et al., 1992), the ventral tegmentalarea (Johnson and North, 1992), and the nucleus accumbens (Yuanet al., 1992).

Within the MSDB the GABAergic neurons inhibited by µ-opioids could belong to the subpopulation of GABAergic neurons that containsthe Ca²⁺-binding protein parvalbumin and projects to the hippocampus (Freund,1989) and/or to the second subpopulation that does not projectoutside of the nucleus. Because we observed a µ-opioid-induceddecrease in local synaptic activity in slices that contained onlythe MSDB, we concluded that the µ-opioid-inhibited MSDB GABAergicneurons make numerous local circuit connections. Anatomically,the presence of such local connections has been much speculatedabout because parvalbumin-immunoreactive terminals have been foundaround both parvalbumin-positive and parvalbumin-negative MSDBstructures (Leranth et al., 1992; Gao et al., 1995). The resultsof the present study and our previous studies on the effects ofserotonin and norepinephrine on MSDB neurons (Alreja, 1996; Alrejaand Liu, 1996) provide strong evidence for the presence of suchlocalconnections.

µ-Opioids inhibit septohippocampal GABA neurons

Interestingly, in addition to making local synaptic connections, the results of the present study indicate that opioid-activatedMSDB neurons also project to the hippocampus. This conclusionis based on the results of our antidromic activation studies onseptohippocampal neurons, which indicate that opioids inhibitseptohippocampal neurons. Additionally, the evidence presentedin this study indicates that the opioid agonist-inhibited septohippocampalneurons are most likely GABAergic in nature. This is suggestedby the short antidromic activation latencies of the opioid-responsiveneurons and thus higher mean conduction velocities (mean, 1.83± 0.14 m/sec; range, 1.1-3.2 m/sec). Conduction velocities inthis range have previously been reported to represent the thicklymyelinated, faster-conducting GABAergic fibers (Freund, 1989;Miller and Freedman, 1993). In contrast, the unmyelinated or lightlymyelinated cholinergic SHNs have much slower conducting fibers(<0.3 m/sec). The conclusion, that the opioid-inhibited SHNs areindeed GABAergic in nature is also supported by our anatomicalcolocalization studies using double-immunofluorescence as wellas the mirror colocalization technique (which has absolute specificity)where we found that a small subpopulation (~20%) of parvalbumin-containingneurons expresses the µ-opioid receptor. As mentioned before,parvalbumin is a Ca²⁺-binding protein, that in the MSDB, is expressed exclusively byseptohippocampal GABAergic neurons (Freund, 1989). At the ultrastructurallevel we found that the µ-opioid receptor in MSDB neurons is localizedto the somatic as well as dendritic membranes. The finding thatonly a small subpopulation of parvalbumin-containing MSDB neuronsexpressed the µ-opioid receptor (~20%) corroborates our electrophysiologicalfindings where only a small subpopulation of GABA-type MSDB neuronswere found to be directly inhibited byopioids.

Significance of the findings

An opioid-induced inhibition of septohippocampal GABAergic SHNs is likely to have a significant effect on hippocampal functionas the GABAergic projection neurons of the MSDB innervate almostevery type of hippocampal interneuron (Freund and Antal, 1988).Through this connectivity, electrical stimulation of septohippocampalGABAergic afferents has been shown to selectively inhibit hippocampalinhibitory cells and so disinhibit pyramidal cells (Toth et al.,1997). An opioid-induced inhibition of septohippocampal GABAergicneurons, as was observed in this study, would therefore disinhibita large number of hippocampal GABAergic neurons and increase bothfeedback and feedforward type of local hippocampal inhibition(Freund and Antal, 1988). The resultant decrease in pyramidalcell excitability could decrease the likelihood for the inductionof long-term potentiation (LTP) because LTP can be preferentiallyinduced when the cells are maximally stimulated (Pavlides et al.,1988). Such effects could therefore explain the memory impairmentthat is observed after intraseptal injections of opioids (seeintroductory remarks). The results of the present study also showthat opioids by decreasing the release of GABA would result ina disinhibition of a subpopulation of cholinergic neurons. Whetherthis disinhibition is opposed by any direct inhibitory effectsof opioids on cholinergic neurons is currently being investigatedin ourlaboratory.

In addition to its impact on septohippocampal circuitry and associated learning and memory-related processes, the µ receptor-mediatedinhibitory effects of opioids in the MSDB may also contributeto the addictive properties of opioids (see introductoryremarks).

In conclusion, the results of the present study suggest that µ- opioids via their actions on MSDB GABAergic neurons are likelyto not only have profound local effects on septal circuitry (byvirtue of a large number of local circuit connections) but wouldalso strongly influence hippocampal function via the septohippocampalpathway.

  FOOTNOTES

Received Sept. 24, 1999; revised Nov. 18, 1999; accepted Nov. 22, 1999.

This work was supported by National Institutes of Health Grants DA09797 to Meenakshi Alreja and NS26068 to Csaba Leranth.We thank N. Margiotta for technical help and Leslie Rosello forhelp in manuscriptpreparation.
Correspondence should be addressed to Meenakshi Alreja, Department of Psychiatry, CMHC 335, Yale University School of Medicine,34 Park Street, New Haven, CT 06508. E-mail: Meenakshi.Alreja{at}yale.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alreja M (1996) Excitatory actions of serotonin on GABAergic neurons of the medial septum and diagonal band of Broca. Synapse 22:15-27[ISI][Medline].
Alreja M, Aghajanian GK (1995) Intracellular diffusion of macromolecules through patch pipettes in brain slices. In: Brain slices in basic and clinical research (Schurr A, Rigor BM, eds), pp 117-130. Boca Raton, FL: CRC.
Alreja M, Liu W (1996) Noradrenaline induces IPSCs in rat medial septal/diagonal band neurons: involvement of septohippocampal GABAergic neurons. J Physiol (Lond) 494:201-215[ISI][Medline].
Baldino Jr F, Beckman AL (1982) An analysis of the origins of the cholinergic and non-cholinergic septal projections to the hippocampal formation of the rat. Brain Res 232:247-252[Medline].
Bloom FE, Rossier J, Battenberg ELF, Bayon A, French E, Henriksen SJ, Siggins GR, Segal D, Browne R, Ling N, Guillemin R (1978) $beta$ -endorphin: cellular localization, electrophysiological and behavioral effects. In: Advances in biochemical psychopharmacology (Costa E, Trabucchi M, eds), pp 89-109. New York: Raven.
Bostock E, Gallagher M, King RA (1988) Effects of opioid microinjections into the medial septal area on spatial memory in rats. Behav Neurosci 106:643-652.
Bot G, Chahl L (1996) Induction of Fos-like immunoreactivity by opioids in guinea-pig brain. Brain Res 731:45-56[Medline].
Botticelli LR, Wurtman RJ (1982) Septohippocampal cholinergic neurons are regulated transsynaptically by endorphin and corticotropin neuropeptides. J Neurosci 2:1316-1321[Abstract].
Bozarth MA (1983) Opiate reward mechanisms mapped by intracranial self-administration. In: The neurobiology of opiate reward processes (Smith JE, Lane JD, eds), pp 331-359. Amsterdam: Elsevier Biomedical.
Carette B, Poulain P (1982) Postsynaptic inhibitory effects of Met- and Leu-enkephalin on endocrine and adjacent neurones in the preoptic-septal region of the guinea pig. Peptides 3:125-133[Medline].
Cohen GA, Doze VA, Madison DV (1992) Opioid inhibition of GABA release from presynaptic terminals of rat hippocampal interneurons. Neuron 9:325-335[ISI][Medline].
Costa E, Panula P, Thompson HK, Cheney DL (1983) The transsynaptic regulation of the septal-hippocampal cholinergic neurons. Life Sci 32:165-179[Medline].
Couceyro P, Douglass J (1995) Precipitated morphine withdrawal stimulates multiple activator protein-1 signaling pathways in rat brain. Mol Pharmacol 47:29-39[Abstract].
Delfs JM, Kong H, Mestek A, Chen Y, Yu L, Reisine T, Chesselet MF (1994) Expression of mu opioid receptor mRNA in rat brain: an in situ hybridization study at the single cell level. J Comp Neurol 345:46-68[ISI][Medline].
Finley JCW, Lindstrom P, Petrusz P (1981) Immunocytochemical localization of $beta$ -endorphin-containing neurons in the rat brain. Neuroendocrinology 33:28-42[ISI][Medline].
French ED, Siggins GR (1980) An iontophoretic survey of opioid peptide actions in the rat limbic system: in search of opiate epileptogenic mechanisms. Regul Pept 1:127-146[ISI][Medline].
Freund T (1989) GABAergic septohippocampal neurons contain parvalbumin. Brain Res 478:375-381[ISI][Medline].
Freund TF, Antal M (1988) GABA-containing neurons in the septum control inhibitory interneurons in the hippocampus. Nature 336:170-173[Medline].
Gao B, Hornung JP, Fritschy JM (1995) Identification of distinct GABA_A-receptor subtypes in cholinergic and parvalbumin-positive neurons of the rat and marmoset medial-septum diagonal band complex. Neuroscience 65:101-117[ISI][Medline].
Goodman RR, Pasternak GW (1985) Visualization of µ₁ opiate receptors in rat brain by using a computerized autoradiographic subtraction technique. Proc Natl Acad Sci USA 82:6667-6671[Abstract/Free Full Text].
Gorelova N, Reiner PB (1996) Role of the afterhyperpolarization in control of discharge properties of septal cholinergic neurons in vitro. J Neurophysiol 75:695-706[Abstract/Free Full Text].
Griffith WH (1988) Membrane properties of cell types within guinea pig basal forebrain nuclei in vitro. J Neurophysiol 59:1590-612[Abstract/Free Full Text].
Griffith WH, Matthews RT (1986) Electrophysiology of AChE-positive neurons in basal forebrain slices. Neurosci Lett 71:169-174