Cholinergic Excitation of Septohippocampal GABA But Not Cholinergic Neurons: Implications for Learning and Memory

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The Journal of Neuroscience, May 15, 2000, 20(10):3900-3908

Cholinergic Excitation of Septohippocampal GABA But Not Cholinergic Neurons: Implications for Learning and Memory
Min Wu¹, Marya Shanabrough², Csaba Leranth²^,³, and Meenakshi Alreja¹^,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, Connecticut 06508

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The medial septum/diagonal band (MSDB), which gives rise to the septohippocampal pathway, is a critical locus for the mnemoniceffects of muscarinic drugs. Infusion of muscarinic cholinergicagonists into the MSDB enhance learning and memory processes bothin young and aged rats and produce a continuous theta rhythm inthe hippocampus. Intraseptal muscarinic agonists also alleviatethe amnesic syndrome produced by systemic administration of muscarinicreceptor antagonists. It has been presumed, but not proven, thatthe cellular mechanisms underlying the effects of muscarinic agonistsin the MSDB involve an excitation of septohippocampal cholinergicneurons and a subsequent increase in acetylcholine (ACh) releasein the hippocampus. Using a novel fluorescent labeling techniqueto selectively visualize live septohippocampal cholinergic neuronsin rat brain slices, we have found that muscarinic agonists donot excite septohippocampal cholinergic neurons, instead theyinhibit a subpopulation of cholinergic neurons. In contrast, unlabeledneurons, confirmed to be noncholinergic, septohippocampal GABA-typeneurons using retrograde marking and double-labeling techniques,are profoundly excited by muscarine. Thus, the cognition-enhancingeffects of muscarinic drugs in the MSDB cannot be attributed toan increase in hippocampal ACh release. Instead, disinhibitorymechanisms, caused by increased impulse flow in the septohippocampalGABAergic pathway, may underlie the cognition-enhancing effectsof muscarinicagonists.

Key words: theta rhythm; 192IgG; p75 receptor; neurotrophin; acetylcholine; memory; cognition; disinhibition

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Basic and clinical studies have long recognized the importance of cholinergic mechanisms in cognitive functioning (Givensand Sarter, 1997), and drugs that increase synaptic acetylcholinelevels are currently the most used for the treatment of cognitivedeficits associated with CNS disorders such as Alzheimer's disease,albeit, with limited effectiveness (Benzi and Moretti, 1998).The septohippocampal (SH) pathway, which originates in the medialseptum/diagonal band (MSDB) and shows progressive degenerationin Alzheimer's disease (Whitehouse et al., 1982), has specificallybeen implicated in cognitive mechanisms. Lesions of the fimbria-fornix,which conveys SH cholinergic (Lewis and Shute, 1967) and GABAergicfibers to the hippocampus (Kohler et al., 1984; Freund, 1989),interfere both with learning and memory tasks and with generationof the theta rhythm in rats (Brito and Brito, 1990). These deficitscan be attenuated by grafting ACh-producing cells to the hippocampus(Dunnett et al., 1982; Dickinson-Anson et al., 1998).

Cholinergic mechanisms operating within the MSDB are also critical for learning and memory. Thus, infusions of muscarinicagonists directly into the MSDB elicit continuous hippocampaltheta (Monmaur and Breton, 1991; Lawson and Bland, 1993) and facilitatelearning and memory-related behaviors both in young (Givens andOlton, 1990) and aged rats (Markowska et al., 1995). Intraseptalinfusions of muscarinic agonists can also alleviate systemic scopolamine-inducedamnesia, suggesting that the MSDB is a critical locus for themnemonic effects of muscarinic drugs (Givens and Olton, 1995).

In general, it is assumed that improvements in SH pathway-related learning and memory tasks occurs as a result of an increasein hippocampal ACh release (Monmaur and Breton, 1991; Givens andOlton, 1994, 1995; Apartis et al., 1998; Bland and Oddie, 1998;Dickinson-Anson et al., 1998). As such, it has been presumed thatthe memory-enhancing effects of intraseptal-muscarinic agonistsoccur because of increased firing of SH cholinergic neurons (Markowskaet al., 1995; Givens and Sarter, 1997). These assumptions havebeen based on earlier studies that reported a muscarinic receptor-mediatedincrease in firing of SH neurons (Dutar et al., 1983; Lamour etal., 1984), which lead to the hypothesis that ACh, via muscarinicreceptors, has a positive feedback effect on SH cholinergic neurons(Dutar et al., 1983; Lamour et al., 1984; Segal, 1986). However,the SH neurons recorded from in these studies were presumed butnot proven to be cholinergic. A small sample of cholinergic-typeMSDB neurons (n = 3), classified using electrophysiological characteristics,were found to be inhibited by muscarine (Serafin et al., 1996).Additional effects of muscarine, such as a block of late afterhyperpolarization(Sim and Griffith, 1991) and decrease in glutamate transmission(Sim and Griffith, 1996) have also been reported in unidentifiedbasal forebrain neurons. Effects of muscarinic agonists on identifiedseptohippocampal cholinergic neurons have not beeninvestigated.

In the present study, we used a novel fluorescent marker, Cy3-192IgG, to selectively label live rat SH cholinergic neuronsand studied their response to cholinergic drugs using extracellularand whole-cell recordings in brain slices. Cy3-192IgG is preparedby conjugating the inert fluorochrome, Cy3, with an antibody againstthe p75 neurotrophin receptor. When injected intraventricularly,Cy3-192IgG retrogradely labels only p75 receptor-expressing neurons(Hartig et al., 1998), which in the MSDB are exclusively cholinergic(Batchelor et al., 1989; Sobreviela et al., 1994). The goal ofthis study was to determine whether identified SH cholinergicneurons are excited by their own neurotransmitter via muscarinicreceptors.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Retrograde labeling of septohippocampal neurons. Young adult male Sprague Dawley albino rats (14- to 21-d-old) were anesthetizedusing the following cocktail: ketamine, 75 mg/kg; xylazine, 4mg/kg, and acepromazine, 0.075 mg/kg. Retrograde labeling of septohippocampalneurons (SHNs) was performed by pressure injecting 50-100 nl ofrhodamine-labeled fluorescent latex microspheres (Lumafluor, Naples,FL) at several sites within the hippocampus of 14- to 21-d-oldrats using a glass micropipette (40-50 µm tip diameter). Rhodaminemicrospheres (0.02-0.2 µm diameter) show little diffusion andconsequently produce small, sharply defined injection sites. Oncetransported back to neuronal somata, the label persists for atleast 10 weeks in vivo and 1 year after fixation. Microsphereshave been reported to possess no obvious cytotoxicity or phototoxicity,as assessed by intracellular recording and staining of retrogradelylabeled cells in brain slice preparation (Katz et al., 1984).The stereotaxic coordinates were: anteroposterior, $-$ 2.8, $-$ 1.4, $-$ 2.8; lateral, $-$ 4, $-$ 1.4, $-$ 2.8; and ventral, $-$ 5.8, $-$ 4.5, $-$ 3.5 to $-$ 6 mm track). Two or more days later, the injected rats were usedto prepare brain slices. Injection sites were confirmed for eachexperiment.

Labeling of septohippocampal cholinergic neurons using Cy3-192IgG. In anesthetized rats Cy3-192IgG (3-5 µl; 0.4 mg/ml) wasstereotaxically injected unilaterally or bilaterally into thelateral ventricle of each rat with a Hamilton syringe (22 gaugeneedle) at a rate of 0.5 µl/min. The coordinates used were: 0.8mm posterior from bregma, 1.2 mm lateral from midline, and 3-4mm below the dura. Two to five days later, slices were preparedfrom Cy3-192IgG-injected rats and used for electrophysiologicalrecordings. Recordings from unlabeled neurons were restrictedto animals injectedbiventricularly.

Colocalization studies. Brain tissue taken from Cy3-192IgG-injected rats was immersion-fixed and, then, consecutive 50 µmsections of the MSDB were cut on a Vibratome. Alternate sectionswere immunostained for either choline acetyltransferase (ChAT)or the calcium-binding protein, parvalbumin (Parv). For the ChATimmunoreaction, the sections were incubated in a rat-anti-ChATprimary antibody (1:5 dilution in PB; Boehringer Mannheim, Indianapolis,IN) overnight at room temperature. Subsequently, sections wereincubated in rabbit anti-rat IgG-fluorescein-labeled (1:100 inPB; Vector Laboratories, Burlingame, CA; FI4000) for 2 hr at roomtemperature in the dark. For Parv, the sections were incubatedin a rabbit anti-Parv (1:500 dilution in PB; gift of K. G. Baimbridge,Vancouver, Canada; overnight at room temperature) followed bygoat anti-rabbit IgG-fluorescein (1:100 in PB; Vector Laboratories;FI1000; 2 hr at room temperature in thedark).

Immunofluorescence was visualized under an Olympus BX50WI scope (Olympus Optical, Tokyo, Japan) using the appropriate filtersfor Cy3 and fluorescein. Cy3 appeared as granules within the cytoplasmof the cells, whereas the ChAT and Parv immunofluorescence washomogeneously distributed in the cells. This made it easy to confirmcolocalization of the two substances in the samecell.

Slice preparation for electrophysiological recordings. Brain slices containing the MSDB were prepared from young adult maleSprague Dawley albino rats (2- to 4-weeks-old) using methods detailedpreviously (Alreja and Liu, 1996). Briefly, rats were anesthetizedwith chloral hydrate (400 mg/kg, i.p.) and killed by decapitation.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, the brain wasremoved and placed in a Petri dish containing ACSF and trimmedto yield a small block containing the MSDB. Coronal slices of~300 µm thickness containing the MSDB were cut with a vibrating-knifemicrotome (Frederick Haer, Bowdingham, ME) and transferred toa Plexiglas recording chamber (1.5 ml volume) on the fixed stageof an Olympus BX50WI scope. The slice was kept in place with agrid and maintained at 33 ± 0.5°C. One to two hours later theslice was used for recording. The chamber was continuously perfusedwith normal ACSF at a rate of 1-2 ml/min.

Fluorescence and infrared imaging. Infrared, differential interference contrast imaging (IR-DIC) (Dodt and Zieglgansberger,1990; Stuart et al., 1993) was performed to visualize neuronsfor extracellular or patch-clamp recording using an Olympus OpticalBX-50 microscope equipped with a 60× water immersion objective(numerical aperture, 0.9; Olympus). Images were detected witha CCD-300-RC camera (DAGE-MTI, Michigan City, IN) and displayedon a standard black and white video monitor (DAGE-MTI, HR 120).The images were transferred to the hard disk of a personal computerusing an LG-3 scientific frame grabber (Scion Image, Frederick,MD) and processed further with Adobe Photoshop. Cy3-192IgG-labeledand rhodamine-labeled neurons were visualized using the appropriatefluorescence filters, as was Lucifer yellow. A neuron viewed withinfrared optics was considered to be the same as that viewed withfluorescence optics when the infrared image and the fluorescentimage of the neuron had the same position and orientation withthe two imagingsystems.

Electrophysiology recordings. The image of the cells in the slice was displayed on a video monitor, and glass pipettes usedfor electrophysiological recordings were visually advanced throughthe slice to the surface of the cell from which recordings weremade. Extracellular recordings were performed with glass micropipettesfilled with 2 M NaCl (5-10 M $Omega$ ). Whole-cell patch-clamp recordingswere performed using previously described methods (Alreja andLiu, 1996). In brief, low-resistance (2.5-3.5 M $Omega$ ) patch pipetteswere filled with a solution containing (in mM): K methylsulfonate/KCl,120; HEPES, 10; BAPTA K₄, 5; sucrose, 20; CaCl₂, 2.38; MgCl₂,1; K₂ATP, 1 and GTP, 0.1, pH 7.32-7.35. All recordings were madeusing an Axoclamp-2B amplifier (Axon Instruments, Foster City,CA) in the bridge mode; the output signal was filtered at 10 kHz.The cells selected for study had spike amplitudes of 70-100 mV.Spike durations were measured at half-spike amplitude. In spontaneouslyfiring cells these measurements were done at the resting potentialand in quiescent cells, firing was evoked by injecting a smallamount of depolarizing current. Voltage-clamp recordings wereperformed using the continuous single-electrode voltage-clampmode. The firing rate, current, and voltage signals were amplifiedand continuously recorded on a chart recorder (Gould 2200). Forintracellular labeling studies, Lucifer yellow (1%) was addedto the patch pipettesolution.

Double-labeling studies. To determine the phenotype of cells recorded with Lucifer yellow-containing patch pipette solutions,double-labeling studies were performed on slices fixed using 4%paraformaldehyde solution. For the ChAT immunoreaction, the sectionswere incubated in a rat anti-ChAT primary antibody (1:5 dilutionin PB; Boehringer Mannheim) overnight at room temperature. Subsequently,sections were incubated in rabbit anti-rat IgG, Texas Red-labeled(1:100 in PB; Vector Laboratories) for 2 hr at room temperaturein thedark.

Materials. Acetylcholine chloride, muscarine chloride, atropine sulfate, and ( $-$ )-scopolamine hydrobromide were obtained fromResearch Biochemicals (Natick, MA). All drugs were diluted inACSF from previously prepared stock solutions that were preparedin water and stored at $-$ 20°C. Rhodamine microspheres were obtainedfrom Lumafluor (Naples, FL), and Cy3-192IgG was custom-synthesizedby Advanced Targeting Systems (San Diego,CA).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Muscarinic agonists excite retrogradely labeled septohippocampal neurons

As mentioned above, antidromically activated SHNs have been shown to be excited by muscarinic receptor agonists both in vivo(Dutar et al., 1983; Lamour et al., 1984) and in vitro in a concentration-dependentand atropine-sensitive manner (Liu et al., 1998). The phenotypeof the excited neurons, while presumed to be cholinergic, hasactually never been confirmed (Lamour et al., 1984). Before initiatingstudies on identified septohippocampal cholinergic neurons, weused a second technique, the technique of retrograde labelingto confirm the effects of muscarine on unidentified SHNs. Extracellularrecordings were performed in retrogradely marked SHNs in rat brainslices prepared from rats in which the retrograde tracer, rhodaminemicrospheres, was injected directly into the rat hippocampus (Fig.1A). ACh (1 mM) and/or muscarine (1-10 µM) produced a profoundexcitatory effect in 8 of 13 SHNs tested (Fig. 1B), which resultedin a 31-300% increase in firing rate (mean, 138 ± 42%). Theseneurons had basal firing rates of 9.1 ± 2.2 Hz (range, 2-19 Hz);ACh/muscarine produced a statistically significant increase inrate (p < 0.001; mean, 16.3 ± 2.5 Hz; range, 8-25 Hz). Four of13 SHNs tested in this study did not respond to muscarine, andone was inhibited by muscarine. All effects of ACh-muscarine wereblocked by the muscarinic receptor antagonist atropine (100 nMto 3 µM). As expected, both the lower and the higher concentrationsof the antagonists blocked the ACh-muscarine responses; the higherconcentrations however, had a much more rapid effect. These observationsthus confirm earlier studies that have reported the presence ofmuscarine-excited MSDB neurons that project to the hippocampus.

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Figure 1. Retrogradely labeled rat septohippocampal neurons are excited by the muscarinic cholinergic receptor agonist muscarine. A1 shows an SHN that was retrogradely labeled using rhodamine beads. A2, The cell was filled with Lucifer yellow during an in vitro whole-cell recording. Note the patch pipette in the right side of the field. B, Chart record shows that a near-maximal concentration (Liu and Alreja, 1997) of bath-applied muscarine (musc) produces a profound and prolonged increase in firing rate in an SHN. Atropine, a muscarinic receptor antagonist, rapidly blocked the response to a subsequent application of muscarine; a high concentration of atropine was used primarily to get a rapid block. Lower concentrations (100 nM) also block ACh-muscarine responses, albeit, with a slower time course.

Cy3-192IgG selectively labels septohippocampal cholinergic neurons in the MSDB

To test the effect of muscarine on identified septohippocampal cholinergic neurons, we injected rats, intraventricularly,with the novel fluorescent marker, Cy3-192IgG. Cy3-192IgG selectivelylabels septohippocampal cholinergic neurons in the MSDB (Hartiget al., 1998).

Before initiating electrophysiological recordings, we performed double-labeling studies to confirm the selectivity of Cy3-192IgGas a marker for cholinergic neurons in the MSDB. Two to five daysafter unilateral or bilateral intraventricular injections of Cy3-192IgG,retrogradely labeled, red-fluorescent neurons could be observedin the MSDB. Consistent with published findings, Cy3-192IgG-labeledMSDB neurons were found to colocalize the enzyme ChAT, a wellestablished marker of cholinergic neurons (Fig. 2A); all cholinergicneurons however did not get labeled with Cy3-192IgG, presumablybecause of incomplete diffusion of Cy3-192IgG (Hartig et al.,1998). In addition, we performed double-labeling studies usingan antibody against the calcium-binding protein parvalbumin. Inthe MSDB, parvalbumin is selectively contained in septohippocampalGABA neurons (Freund, 1989). We found that parvalbumin-positiveneurons never colocalized Cy3-192IgG (Fig. 2B). As expected, Cy3-192IgG-labeled neurons also did not colocalize the enzyme glutamic aciddecarboxylase (GAD); which is expressed both by local as wellas by projection GABAergic neurons (data not shown). Thus, theselectivity of Cy3-192IgG for cholinergic neurons is similar tothat reported for the well-established immunotoxin 192IgG-saporin(Wenk et al., 1994; Wiley et al., 1995).

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Figure 2. Double-labeling studies confirm that Cy3-192IgG selectively labels septohippocampal cholinergic and not GABAergic neurons. A shows a Cy3-192IgG-retrogradely labeled neuron (A1) that is ChAT-positive (A2) and therefore confirmed to be cholinergic. B shows a Cy3-192IgG-labeled neuron (B1) that does not colocalize the calcium-binding protein parvalbumin (B2; Parv), a marker of septohippocampal GABA neurons. Note that a parvalbumin-positive neuron in the same field is not labeled with Cy3-192IgG.

Therefore, although the Cy3-192IgG-labeled neuronal population in the MSDB is exclusively cholinergic, the unlabeled populationalthough primarily GABAergic (local and projection), also includesunlabeled cholinergic neurons. With these findings in view, wetested the effects of muscarinic agonists on both Cy3-192IgG-labeledand unlabeledneurons.

Muscarine does not excite Cy3-192IgG-labeled MSDB neurons but profoundly excites unlabeled MSDB neurons

Extracellular and whole-cell recordings were made from Cy3-192IgG-labeled and unlabeled MSDB neurons visualized in rat brainslices using an IR-DIC videomicroscope equipped with appropriatefilters for visualization of fluorescence. Cy3-192IgG-labeledneurons appeared as red fluorescent neurons with a punctate-typestaining (Fig. 3), presumably because of clustering of the redfluorescent antibodies in compartments resembling lysosomes (Hartiget al., 1998). Cy3-192IgG-labeled neurons had a healthy appearance(Fig. 3); 43% of the neurons from which we recorded (n = 53) firedspontaneously at a rate of 2 ± 0.07 Hz recorded extracellularly.Whole-cell recordings were also established in 37 of 53 neuronstested. These neurons exhibited electrophysiological characteristicssimilar to those described for cholinergic neurons using double-labelingtechniques by previous workers (see below).

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Figure 3. Visualization of septohippocampal cholinergic neurons in live rat brain slices using Cy3-192IgG, a selective marker of p75-receptor-expressing neurons in the MSDB. A, Cy3-192IgG-labeled neurons show a granular fluorescent labeling as seen in a 300-µm-thick slice preparation. B, The same neurons visualized using differential interference contrast, infrared videomicroscopy. Note an unlabeled neuron (arrow) and the healthy appearance of the labeled cells.

The effect of ACh and/or the muscarinic receptor agonist, muscarine (1-10 µM) was tested in a total of 47 Cy3-labeled neurons.Surprisingly, none of the Cy3-192IgG-labeled neurons tested wereexcited by ACh-muscarine, although they were strongly excitedby the excitatory amino acid glutamate (n = 18; data not shown).Instead, muscarine produced inhibitory responses (Fig. 4A) in62% (29 of 47) of the Cy3-labeled neurons (1-10 mV hyperpolarization;mean, 3.5 ± 0.6 mV). The remaining 38% neurons were not affectedby muscarine.

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Figure 4. Cy3-192IgG-labeled neurons are not excited by muscarine, but unlabeled neurons are strongly excited by muscarine. A, Response of a Cy3-192IgG-labeled neuron to depolarizing and hyperpolarizing current steps (step size, 0.02 nA; maximum step, +0.04 nA). Note the presence of inward rectification that is characteristic of cholinergic neurons. Chart record shows that this spontaneously firing neuron (2 Hz) responded to muscarine with a 80% decrease in firing rate. Inhibitory responses were observed in ~60% of Cy3-192IgG-labeled neurons, none of the neurons were excited by muscarine. B shows the response of an unlabeled MSDB neuron that responded to ACh, with a 600% increase in firing rate. Note that a second application of ACh produced a similar response; the excitatory effect was rapidly blocked by the muscarinic receptor antagonist atropine, which was used at a high concentration in this cell so as to get a fast blockade of the ACh response. Similar excitatory responses to ACh-muscarine were observed in 91% of the unlabeled neurons tested. Also note the different electrophysiological profile of this neuron as compared to the Cy3-192IgG-labeled neuron shown above. Specifically, note the presence of a depolarizing sag in response to hyperpolarizing pulses (step size, 0.02 nA; maximum step, +0.04 nA). C, Bar chart summarizes the effect of muscarine on Cy3-labeled and unlabeled neurons. Note that although none of the Cy3-labeled neurons were excited by muscarine, 91% of unlabeled neurons responded to the agonists with an excitation. D, Bar chart shows that whereas muscarine produced a significant decrease in firing rate in Cy3-labeled neurons, it produced an increase in rate in unlabeled neurons.

In sharp contrast to the effects of ACh-muscarine on Cy3-192IgG-labeled neurons, 91% of the unlabeled neurons (31 of 34) wereprofoundly excited by ACh-muscarine (Fig. 4B) and showed a 19-600%increase in firing rate (mean, 192 ± 36%). These neurons had basalfiring rates of 4.2 ± 0.5 Hz (range, 0.6-11.5 Hz); ACh-muscarineproduced a statistically significant increase in rate (p < 0.001;mean, 11.3 ± 0.9 Hz; range, 1.7-25 Hz). Two neurons were not affectedby ACh-muscarine, whereas one neuron was inhibited. These dataare summarized in Figure 4, C and D. Consistent with previousobservations, repeated applications of ACh-muscarine had a similareffect and did not show any desensitization (Liu et al., 1998).

All effects of ACh-muscarine, both excitatory and inhibitory, in labeled and unlabeled neurons, were blocked by the muscarinicreceptor antagonists, atropine, or scopolamine (100 nM to 3 µM;n =8).

Thus, the sampled Cy3-192IgG neuronal population discussed above, which is exclusively cholinergic, was found never to beexcited by muscarine. This raises an important issue: if the septohippocampalneurons that are excited by muscarine are not cholinergic, thenwhat is their phenotype? As mentioned before, a subpopulationof GABA neurons in the MSDB also projects to the hippocampus viathe fimbria-fornix.

Muscarine-excited MSDB neurons are noncholinergic, septohippocampal GABA-type

The GABA neurons that project to the hippocampus from the MSDB are distinct from other neurons in the MSDB (cholinergic andlocal GABA) in that they exclusively express the calcium-bindingprotein parvalbumin (Freund, 1989). Because of this unique property,parvalbumin has become a well established marker of septohippocampalGABA neurons in the MSDB (Gao et al., 1995; Leranth and Vertes,1999). Parvalbumin-containing neurons in the cortex (Kawaguchiand Kubota, 1997), hippocampus (Sik et al., 1995), and more recentlyin the MSDB (Morris et al., 1999), have been shown to possessunique spiking properties, such as a lack of spike frequency accommodationand thus an ability to fire rapidly; properties that may be reflectiveof the calcium-buffering properties of parvalbumin. Additionally,in the MSDB, parvalbumin-positive neurons have been reported tobe spontaneously firing, possess short duration spikes (0.3-0.7msec), and exhibit a depolarizing sag in response to a hyperpolarizingcurrent.

To determine if muscarinic agonists excite MSDB neurons possessing electrophysiological characteristics of parvalbumin-positiveneurons (and therefore of septohippocampal GABA-type neurons),we performed whole-cell recordings in brain slices taken fromnoninjected rats and noted the effect of muscarinic agonists onMSDB neurons that clearly exhibited the abovementioned electrophysiologicalcriteria of parvalbumin-positive neurons. Of the 16 MSDB neuronsso characterized, 14 were found to respond to muscarinic agonistswith a profound excitation (Fig. 5A). These neurons had basalfiring rates of 5.6 ± 1 Hz (range, 1-18 Hz), which increased to17-25 Hz after application of muscarine (p < 0.001; n = 5). Oneneuron was inhibited by muscarine. In eight neurons, the effectof muscarine was tested under voltage clamp at a holding potentialof $-$ 60 mV, muscarine produced a 50-80 pA inward current in theeight neurons tested (mean, 52.5 ± 0.7 pA; data not shown). Thus,similar to unlabeled neurons above, muscarinic agonists were foundto excite a vast majority of parvalbumin-type MSDB neurons (87.5%).

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Figure 5. Septohippocampal GABA-type but not cholinergic-type neurons rats are excited by muscarine. A, These whole-cell recordings were performed in brain slices taken from uninjected rats. Neurons were classified as septohippocampal cholinergic-type or GABA-type based on electrophysiological characteristics (see Results). A1 shows a fast-spiking, nonaccommodating, GABA-type MSDB neuron. A2, Chart recording from the same neuron shows the profound excitatory effect of bath-applied muscarine. An excitatory effect was observed in 87.5% of septohippocampal GABA-type neurons tested. Note the depolarizing sag in response to the hyperpolarizing pulses and the presence of an anode-break excitation after termination of the hyperpolarizing pulses. B, Whole-cell recording from a spontaneously firing cholinergic-type MSDB neuron. This cell exhibited a prominent slow afterhyperpolarization after a spike and strong inward rectification in response to hyperpolarizing pulses. Bath-applied muscarine (10 µM, 2 min) produced a 9 mV hyperpolarization that reversed after washout (washout not shown). Inhibitory effects of muscarine were observed in 62.5% of cholinergic-type MSDB neurons. C, Bar chart summarizes the effect of muscarine on cholinergic- and parvalbumin-type MSDB neurons. Note that although none of the ChAT-type neurons were excited by muscarine, 88% of Parv-type neurons responded to the agonists with an excitation. D, Bar chart shows that whereas muscarine produced a significant decrease in firing rate in ChAT-type neurons, it produced an increase in rate in Parv-type neurons.

Again, in contrast, to the parvalbumin-containing, septohippocampal GABA-type neurons, neurons exhibiting electrophysiologicalproperties of cholinergic-type neurons (also recorded from slicestaken from noninjected rats), were found never to be excited bymuscarine. Cholinergic-type neurons in uninjected rats thereforeresponded to muscarine in a manner similar to the Cy3-192IgG-labeledpopulation described above. Whereas 10 of 16 (62.5%) cholinergic-typeneurons were inhibited by muscarine (1-10 mV hyperpolarization),the remaining six neurons were not affected by muscarine (Fig.5B). Sixty percent of the neurons were spontaneously firing (range,0.1-2 Hz; mean, 1.2 ± 0.2 Hz). The electrophysiological criteriaused for identification of cholinergic-type MSDB neurons includedthe presence of a prolonged spontaneous afterhyperpolarization(200-700 msec) after a single spike and presence of anomalousrectification but no depolarizing sag in response to hyperpolarizingpulses; these criteria were based on those described by earlierworkers (Griffith and Matthews, 1986; Markram and Segal, 1990;Gorelova and Reiner, 1996). The data on cholinergic-type and parvalbumin-typeneurons is summarized in Figure 5, C and D.

The effect of the muscarinic agonist was also tested in presence of tetrodotoxin (TTX). Whereas the excitatory response tomuscarine persisted in presence of TTX in all six neurons tested,the inhibitory response in cholinergic-type neurons was blockedby TTX in two of five neurons tested (data not shown). In boththese neurons the TTX-sensitive muscarinic inhibition was accompaniedby an increase in the frequency of inhibitory synaptic activity,which is both TTX- and bicuculline-sensitive (Kumar et al., 1997).Thus, cholinergic-type neurons in the MSDB exhibited both directpostsynaptic as well as indirect inhibitoryresponses.

To further confirm the noncholinergic phenotype of the neurons excited by muscarine, we labeled MSDB neurons with Luciferyellow during whole-cell recordings and, after completion of theexperiment, we performed double-labeling studies using an antibodyagainst the enzyme ChAT, which is a well established marker ofcholinergic neurons. Of the eight successfully double-labeledneurons, five were excited by muscarine, and the remaining threewere not affected. Interestingly, the five neurons that were excitedby muscarine were all found to be ChAT-immunonegative, supportingthe above findings that suggested that the neurons excited bymuscarine are noncholinergic. All the ChAT-immunonegative neuronshad electrophysiological properties similar to those that havebeen described for septohippocampal GABA neurons (see above).Of the three neurons that were not affected by muscarine, onecolocalized ChAT, and two were ChAT-immunonegative.

In conclusion, septohippocampal cholinergic neurons were never found to be excited by muscarine, whereas noncholinergic, septohippocampalGABA-type neurons were profoundly excited bymuscarine.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The main findings of this study are: (1) muscarinic receptor agonists do not excite septohippocampal cholinergic neurons,and (2) noncholinergic, septohippocampal GABA-type MSDB neuronsare strongly excited by muscarinic agonists. These findings, therefore,challenge the current belief that MSDB cholinergic neurons areexcited by their own neurotransmitter and that this excitationand the subsequent increase in hippocampal ACh underlies the improvementin learning and memory that is observed after intraseptal administrationof muscarinicdrugs.

Muscarinic agonists do not excite septohippocampal cholinergic neurons

Using a fluorescent labeling technique, involving the p75-receptor antibody conjugated to the Cy3 fluorochrome for selectivevisualization of septohippocampal cholinergic neurons locatedin the MSDB, we have found no excitatory effects of muscarineon Cy3-192IgG-labeled septohippocampal cholinergic neurons. Infact, Cy3-labeled septohippocampal cholinergic neurons are eitherinhibited or not affected by muscarine. Recordings from cholinergic-typeMSDB neurons (in brain slices prepared from noninjected rats),classified according to previously published electrophysiologicalcriteria, also yielded the same results. Therefore, the presenceof Cy3-192IgG in septohippocampal cholinergic neurons does notappear to alter their responsivity to muscarinic agonists. Theelectrophysiological properties of Cy3-labeled neurons were alsosimilar to those of cholinergic-type neurons recorded from noninjectedrats, suggesting that Cy3-192IgG may be a useful tool worthy ofbeing exploited for future studies on septohippocampal cholinergicneurons as well as on p75 receptor-expressing neurons elsewherein the brain, such as in the nucleusbasalis.

The finding that septohippocampal cholinergic neurons are not excited by muscarine is very interesting because intaseptalinjections of muscarinic agonists elicit continuous hippocampaltheta rhythm and produce behavioral improvements in working andmemory tasks both in young and aged rats (see introductory remarks).Our results indicate that the mechanisms underlying intraseptalmuscarinic agonist-induced improvements in learning and memoryand production of theta rhythm do not involve an impulse-dependentincrease in hippocampal ACh release. This conclusion is supportedby the findings of microdialysis studies that show that infusionsof muscarinic agonists into the MSDB produce a dose-dependentdecrease in hippocampal ACh release (Gorman et al., 1994) or haveno effect (Moor et al., 1995). A decrease in hippocampal ACh releasewould be predicted by the results of the present study because60-65% of septohippocampal cholinergic neurons from which we recordedwere found to be inhibited bymuscarine.

The finding that a subpopulation of septohippocampal cholinergic neurons is inhibited by muscarine is consistent with light-microscopiccolocalization studies that have demonstrated the presence ofm2 receptor immunoreactivity (a muscarinic receptor associatedwith inhibitory responses) in a subset of choline acetyltransferase-immunoreactiveas well as noncholinergic neurons (Van der Zee and Luiten, 1994;Levey et al., 1995) and retrogradely labeled septohippocampalneurons (Rouse and Levey, 1996). m2 receptor mRNA has also beenshown to colocalize with cholinergic MSDB neurons (Vilaro et al.,1992).

Muscarinic agonists excite noncholinergic, septohippocampal GABA-type neurons

The finding that muscarinic agonists do not have any excitatory effects on septohippocampal cholinergic neurons raises thequestion of what cellular mechanism or mechanisms might mediatethe effects of intraseptal muscarinic drugs on learning and memoryand the associated theta rhythm. The results of the present studyas well as previously published studies clearly show that muscarine-excitedMSDB cells do project to the hippocampus (Dutar et al., 1983;Lamour et al., 1984; Liu et al., 1998), suggesting then that themuscarine-excited neurons must then be GABAergic. As mentionedpreviously, similar to the cholinergic neurons, the septohippocampalGABA neurons also project to the hippocampus via the fimbria-fornix.In fact, in our earlier study using the technique of antidromicactivation, we found that septohippocampal neurons excited bymuscarine had fast-conducting fibers, with conduction velocitiesgreater than 1 m/sec, which may be suggestive of GABA neurons(Liu et al., 1998).

In the present study, muscarinic agonists consistently produced a strong excitation of unlabeled neurons in Cy3-192IgG-injectedrats, some of which were confirmed to be noncholinergic usingthe technique of double labeling. Because Cy3-192IgG does notlabel parvalbumin-positive or GAD-positive neurons of the MSDB,it is likely that the unlabeled cell population, which was profoundlyexcited by muscarine, included the septohippocampal GABA neuronsof the MSDB. Additionally, in uninjected rats a vast majorityof neurons exhibiting electrophysiological properties characteristicof septohippocampal GABA-type neurons were profoundly excitedbymuscarine.

Implications of the findings

The present study suggests that an activation of septohippocampal GABA neurons and not septohippocampal cholinergic neuronsmay underlie the behavioral and electrophysiological effects observedafter intraseptal infusions of muscarinic agonists in rats. Whereasmost published research has focused on the importance of septohippocampalcholinergic mechanisms in learning and memory functions and ingeneration of the theta rhythm, the role of septohippocampal GABAergicmechanisms is being increasingly recognized, especially with regardto production of theta activity (Stewart and Fox, 1990; Bassantet al., 1995; Brazhnik and Fox, 1997, 1999; Monmaur et al., 1997).The results of the present study suggest that the reported effectsof intraseptal carbachol on theta rhythm (Monmaur and Breton,1991; Lawson and Bland, 1993) cannot be attributed to an increasein firing of septohippocampal cholinergic neurons. Therefore,the question is, how important are the cholinergic neurons forcarbachol-induced generation of theta rhythm? Buzsaki's laboratoryhas demonstrated that intraseptal infusions of carbachol continueto elicit theta activity in the hippocampus even in the completeabsence of MSDB cholinergic neurons in 192IgG-saporin-treatedrats, albeit, at a reduced amplitude, thereby indicating a criticalrole of septohippocampal GABAergic neurons in generation of thetarhythm (Lee et al., 1994).

Anatomically, the septohippocampal GABA neurons are well positioned to exert indirect but strong effects on hippocampal pyramidalneurons. In contrast to the septohippocampal cholinergic neurons,which innervate almost every type of neuron in the hippocampus(pyramidal cells, dentate granule cells, inhibitory interneurons)(Frotscher and Leranth, 1985), the septohippocampal GABA neuronsselectively innervate only the GABA interneurons of the hippocampus(Freund and Antal, 1988). Via this very selective connectivity,the septohippocampal GABA neurons can theoretically produce apowerful disinhibitory effect on hippocampal pyramidal neurons.In fact, a recent study performed using a novel combined septohippocampalslice preparation has provided electrophysiological evidence thatactivation of septohippocampal GABAergic fibers can lead to adisinhibition of pyramidal cells (Toth et al., 1997). Therefore,it is conceivable that a profound muscarinic agonist-induced excitationof septohippocampal GABA neurons, as was observed in the presentstudy, could, via hippocampal interneurons, produce a powerfuldisinhibition of pyramidal cells and possibly promote inductionof long-term potentiation in the hippocampus. Long-term potentiationis preferentially induced when the pyramidal cells are maximallystimulated (Pavlides et al., 1988).

In addition to muscarinic agonists, serotonin, primarily via 5-HT_2A receptors, (Alreja, 1996; Liu et al., 1997), and norepinephrine,via $alpha$ ₁ receptors (Alreja and Liu, 1996), also excite septohippocampalGABA neurons, albeit, not as profoundly as muscarine. Opioids,on the other hand, via mu receptors, inhibit septohippocampalGABA neurons (Alreja et al., 2000). Interestingly, behavioralstudies have reported that intraseptal infusions of opioids (Bostocket al., 1988; Ragozzino et al., 1992) or $alpha$ ₁ noradrenergic receptorantagonists (Marighetto et al., 1989), treatments that would decreaseimpulse flow in the septohippocampal GABA pathway, impair learningandmemory.

Pharmacologically, the excitatory effects of muscarinic agonists on septohippocampal neurons are mediated via non-M₁ typemuscarinic receptors (M₃ and possibly M₅ subtypes) (Liu et al.,1998). Thus, muscarinic agonists directed toward the M₃ and M₅receptor subtypes, could, theoretically by mimicking the behavioraleffects of muscarine, alleviate age-related amnesia as age-relatedamnesia, and decrease in theta power can be alleviated by intraseptalinfusions of muscarinic agonists in rats (Markowska et al., 1995).If mechanisms similar to those that occur in aged rats also contributeto dementias associated with Alzheimer's, Parkinsonism, or eventhose associated with mental illnesses such as schizophrenia,then M₃ and M₅-receptor agonists could prove usefultherapeutically.

  FOOTNOTES

Received Nov. 29, 1999; revised March 2, 2000; accepted March 6, 2000.

This work was supported by National Alliance for Research on Schizophrenia and Depression and National Institutes of HealthGrants DA09797 to M.A. and NS26068 to C.L. We thank N. Margiottafor technical help and Leslie Rosello for help in manuscriptpreparation.
Correspondence should be addressed to Dr. Meenakshi Alreja, Department of Psychiatry, CMHC 335A, Yale University School ofMedicine, 34 Park Street, New Haven, CT 06508. E-mail: Meenakshi.Alreja{at}yale.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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