Abstract
The medial septum/diagonal band of Broca complex (MSDB) is a key structure that modulates hippocampal rhythmogenesis. Cholinergic neurons of the MSDB play a central role in generating and pacing theta-band oscillations in the hippocampal formation during exploration, novelty detection, and memory encoding. How precisely cholinergic neurons affect hippocampal network dynamics in vivo, however, has remained elusive. In this study, we show that stimulation of cholinergic MSDB neurons in urethane-anesthetized mice acts on hippocampal networks via two distinct pathways. A direct septo-hippocampal cholinergic projection causes increased firing of hippocampal inhibitory interneurons with concomitantly decreased firing of principal cells. In addition, cholinergic neurons recruit noncholinergic neurons within the MSDB. This indirect pathway is required for hippocampal theta synchronization. Activation of both pathways causes a reduction in pyramidal neuron firing and a more precise coupling to the theta oscillatory phase. These two anatomically and functionally distinct pathways are likely relevant for cholinergic control of encoding versus retrieval modes in the hippocampus.
- acetylcholine
- encoding
- hippocampus
- in vivo electrophysiology
- medial septum
- theta oscillation
Introduction
Neuromodulators such as acetylcholine (ACh) are of central importance in modulating cortical rhythmogenesis and behavior. In the hippocampus, ACh is mainly derived from cholinergic neurons in the medial septum/diagonal band of Broca complex (MSDB) (Mesulam et al., 1983). In this structure, ACh is thought to promote functional network states that allow efficient encoding of novel information. In hippocampal networks, this is achieved by increasing theta activity and synchronization of neurons within and across regions, thus promoting synaptic plasticity (Pavlides et al., 1988; Hyman et al., 2003). At the same time, ACh inhibits recurrent CA3 networks relevant for information retrieval. For example, synaptic transmission from longitudinal association fibers is cholinergically suppressed in vitro (Hasselmo et al., 1995) and ACh release in the hippocampus suppresses sharp-wave ripple events in the CA3 region in vivo (Vandecasteele et al., 2014).
Consistent with this notion, both hippocampal ACh release and hippocampal theta activity are increased during exploration or novelty experience, as well as during arousal or stress (Giovannini et al., 2001; Anzalone et al., 2009; Stanley et al., 2012; for reviews see Bland, 1986; Stewart and Fox, 1990; Buzsáki, 2002; Buzsáki and Moser, 2013). Conversely, lesions of cholinergic MSDB neurons or the septo-hippocampal pathway impair recognition of novel place (Cai et al., 2012) and spatial learning (Berger-Sweeney et al., 2001; Moreau et al., 2008). Moreover, pharmacologically blocking ACh receptors locally in the hippocampal CA3 or CA1 regions disrupts encoding of spatial information while sparing retrieval (Rogers and Kesner, 2003).
The presence of rhythmically bursting cells in the MSDB, initially discovered in rabbits (Petsche et al., 1962; Stumpf et al., 1962), gave rise to the hypothesis that the MSDB serves as a “pacemaker” for the hippocampal theta rhythm. Indeed, lower-frequency theta oscillations (3–6 Hz) during alert immobility and under urethane anesthesia are fully abolished by muscarinic blocker injection into the MSDB (Kramis et al., 1975). However, freely moving animals show a faster theta component that is only partly inhibited by cholinergic blockers (Kramis et al., 1975) or selective lesions of cholinergic MSDB neurons (Lee et al., 1994; Bassant et al., 1995).
When more extensive lesions of either the MSDB or the fimbria-fornix pathway were performed in urethane-anesthetized animals (Andersen et al., 1979) or awake animals (Green and Arduini, 1954; Donovick, 1968; Rawlins et al., 1979), hippocampal theta rhythms were completely abolished. Likewise, global inhibition of MSDB activity in freely moving animals eliminates theta oscillations (Chrobak et al., 1989; Lawson and Bland, 1993; Givens and Olton, 1994). Moreover, combined lesions of both GABAergic and cholinergic neurons abolish theta oscillations, whereas lesioning either system individually causes an incomplete reduction (Yoder and Pang, 2005).
These data suggest that neurons of the MSDB drive hippocampal theta oscillations and that different MSDB systems cooperate to achieve hippocampal modulation. Furthermore, they establish the relevance of the septo-hippocampal system for inducing a hippocampal state that allows the detection of novelty and formation of new memories. How precisely cholinergic neurons affect hippocampal network dynamics in vivo, however, has remained elusive. We show here that cholinergic MSDB neurons generate hippocampal theta rhythm via an MSDB relay. Simultaneously, hippocampal inhibitory interneuron activity is increased, whereas principal cell activity is decreased via direct septo-hippocampal projections. This results in an increased spike-phase coupling of hippocampal principal neurons.
Materials and Methods
Mice.
For optogenetic stimulation experiments, adult homozygous B6;129P2-Pvalbtm1(cre)Arbr/J parvalbumin [PV-IRES-Cre (PV-Cre) knock-in mice; The Jackson Laboratory] or heterozygous B6;129S6-Chattm1(cre)Lowl/J ChAT-IRES-Cre (ChAT-Cre) knock-in mice (The Jackson Laboratory) of both sexes were used. Mice were bred under pathogen-free conditions in an animal facility and maintained on a 12 h light/dark cycle with rodent chow and water ad libitum in groups of two to four animals per cage. Male mice were separated and housed as singles after surgery. All animal experiments were conducted in accordance with the guidelines of the Animal Care and Use Committee of the University of Bonn.
Viral transduction.
We used a recombinant adenoassociated virus (rAAV) of the serotype 2 genome contained in a hybrid serotype 1 and 2 capsid (S2/1) carrying the humanized channelrhodopsin 2 with the H134R mutation (hChR2) (Nagel et al., 2005) fused to the enhanced yellow fluorescent protein (eYFP) in a double-floxed inverted open reading frame under control of the human elongation factor-1α promoter. This rAAV was injected under stereotactic control into the MSDB of ChAT-Cre and PV-Cre mice to achieve specific expression of hChR2-eYFP in cholinergic and GABAergic neurons, respectively. The plasmid (Addgene plasmid 20298) was provided by Karl Deisseroth (Stanford University). For a detailed description of the virus production, see van Loo et al. (2012). For virus injection, mice within an age of 6–10 weeks were anesthetized via an intraperitoneal injection of ketamine (100 mg/kg body weight, WDT, Garbsen, Germany) and medetomidine (1 mg/kg body weight, Domitor; Orion Pharma). Both drugs were diluted in sterile 0.9% sodium chloride solution (Fresenius Kabi) to inject a volume of 100 μl per 10 g body weight. During surgery, mice were kept on a 37°C heating table and eye ointment (Bepanthen; Bayer) was used to prevent corneal drying. Local anesthesia (10% lidocaine, xylocain pumpspray; AstraZeneca) was applied to the skin above the skull before making an incision to expose the skull surface. After scraping away the pericranium, a burr hole was made at a stereotactically identified site above the MSDB (1 mm anterior to bregma, 0.7 mm lateral-right to the midline). Injection was aimed at 2 sites at 4.8 and 4.4 mm ventral to bregma with a 10° polar and −90° azimuth angle. The stereotactic coordinates were obtained from the atlas of Paxinos and Franklin (2008). A total amount of 2 μl viral suspension was injected via a microcontroller (SYS-MICRO4; WPI) operated electrical micropump (UMP3; WPI) at a rate of 100 nl/min through a 34 g bevelled needle (NanoFil; WPI) at the two ventral sites (1 μl at each site). The needle was kept in place for 3 min after injection at the first position and for 5 min after injection at the second position before withdrawal to prevent backflow of the virus. A broadband antibiotic ointment (Polyspectran; Alcon Pharma) was applied to the wound and the skin was sutured using an absorbable antibacterial thread (Coated VICRYLR Plus antibacterial polyglactin 910 5-0 RB10.70 suture; Johnson & Johnson Medical). Buprenorphine hydrochloride (50 μg/kg body weight, B9275; Sigma-Aldrich) for analgesia and atipamezole (5 mg/kg body weight, Antisedan; Orion Pharma) for antagonizing medetomidine were injected intraperitoneally after surgery. Both drugs were diluted in sterile 0.9% sodium chloride solution to inject a volume of 50 and 100 μl per 10 g bodyweight (buprenorphine and medetomidine, respectively). Mice were housed for at least 3 weeks before performing electrophysiological experiments to give them time to recover and to give ChR2 time to accumulate in the cell membrane.
In vivo electrophysiological recordings.
For electrophysiological experiments, mice were anesthetized with two intraperitoneal injections of urethane (catalog no. U2500; Sigma-Aldrich) separated by 30–45 min. The first injection was performed at a concentration of 1.5 g/kg body weight, the second at 0.375 g/kg body weight. The mouse head was fixed in a stereotactic frame (Model 900; David Kopf Instruments) while mice were kept on a heating plate to keep their body temperature stable between 36°C and 37°C throughout the experiment. Body temperature was monitored using a rectal probe. Two hundred microliters of Glucosteril 5% (Fresenius Kabi) were administered subcutaneously every 2 h throughout the experiment. The end of a bare light fiber (0.22 numerical aperture, 550 μm core, BFL22-550; Thorlabs) was implanted with the front aperture just above the MSDB. The fiber tip was advanced 4 mm of radial distance away from the skull surface with a 10° polar and −90° azimuth angle. At the skull surface, the penetration point of the fiber was adjusted to 1 mm anterior to bregma and 0.7 mm lateral-right to the midline. A 1.2 mm major diameter screw (00-96x1/16 mouse screw; Plastics One) was implanted above the cerebellum as a reference electrode. For experiments with focal injections into the MSDB, an additional hole was drilled 1.6 mm anterior to bregma and 0.6 mm lateral-right to the midline for insertion of an injection needle (34 g beveled NanoFil; WPI). The needle was advanced 4.1 mm of radial distance away from the ventral coordinate of bregma at a 10° polar and 45° azimuth angle. This resulted in the needle tip finally positioned at 1 mm anterior and 4.0 mm ventral to bregma exactly at the midline. For experiments with focal injections into the hippocampus, a hole was drilled 0.1 mm posterior to bregma and 2.7 mm lateral-right to the midline. The needle was advanced 2.7 mm from the ventral coordinate of bregma at a 45° polar and 55° azimuth angle. This resulted in the tip finally being positioned at 1.5 mm posterior, 1.6 mm right-lateral, and 1.9 mm ventral to bregma. For insertion of the silicon probe, a cranial window was drilled 1.7 mm posterior to bregma and 1.0–2.2 mm lateral-right to the midline above the dorsal hippocampus. The dura mater was removed and the silicon probe was advanced vertically with the tip at a depth of 2.2 mm from the cortical surface. The closest distance from the tip of the injection needle to the silicon probe shanks was ∼0.2 mm.
The heart rate was monitored and recorded using a steel needle in the skin of the forepaw or hindpaw. In experiments with focal drug application, the microsyringe needle for focal drug injections was carefully advanced in a stepwise manner to the final position just above the MSDB using a microcontroller. Hippocampal field potentials were recorded simultaneously, allowing us to monitor whether the needle insertion itself affected the effects of medial septal optogenetic stimulation. This was never the case if the final location of the needle tip was above the MSDB as described. We did, however, observe strong effects of microinjection needle insertion if it was advanced further into the MSDB (data not shown).
Data acquisition.
The silicon probe (A4x8-5 mm-100-400-413-A32; NeuroNexus) used for in vivo recordings of LFP and single unit activity had 32 electrode contacts, each with a surface area of 413 μm2, distributed on four 15 μm thick shanks, with each shank having eight electrodes vertically distributed with 100 μm spacing. The distance between shanks was 400 μm. Intrahippocampal LFP signals were amplified (100×) and acquired continuously at 48 kHz on a 32-channel recording system with 16-bit resolution (dacqUSB; Axona). For determination of the electrode positions, a microspatula tip of a high molecular weight (500,000 MW) lysine-fixable biotinylated dextran conjugate (catalog no. D-7142; Invitrogen) was dissolved in deionized water and carefully applied to the silicon probe shanks with a small brush before surgery.
Reconstruction of electrode position.
After surgery, the mouse was deeply anesthetized via an intraperitoneal injection of ketamine (100 mg/kg body weight) and xylazine (20 mg/kg body weight) and heart perfusion was performed with 5 ml of Ringer's solution (Fresenius Kabi) at a rate of 2 ml/min while the abdominal aorta was clamped. The brain was removed and stored for 4 d at 4°C in a fixation solution containing 4% methanol-stabilized formalin (catalog no. F1635; Sigma-Aldrich), dissolved in PBS (PBS, catalog no. L 182-10; Biochrom). Fifty-micrometer-thick coronal slices were cut with a vibratome (VT1000S; Leica) in ice-cold PBS solution and subsequently stained with a streptavidin-conjugated green fluorescent dye (Alexa Fluor 488 streptavidin; Invitrogen) diluted 1:500. The track and tip position of the silicon probe shanks were identified and used for electrode position reconstruction, corrected for 5% estimated tissue shrinkage. Data from electrodes for which position could not be determined unambiguously were excluded from further analysis.
Pharmacology.
For systemic intraperitoneal injections of atropine, we used atropine sulfate monohydrate (catalog no. A0257; Sigma-Aldrich) at a concentration of 50 mg/kg body weight. Atropine sulfate monohydrate was dissolved in sterile 0.9% sodium chloride solution at 5 mg/ml to inject a volume of 100 μl per 10 g body weight. For focal injections of atropine into the MSDB, we used atropine sulfate monohydrate at a concentration of 7.2 mm, dissolved in artificial CSF (ACSF) consisting of the following (in mm): NaCl, 125; KCl, 3.5; NaH2PO4, 1.25; NaHCO3, 26; CaCl2, 2; MgCl2, 2; d-glucose, 15 (Sigma-Aldrich). A total volume of 300 nl was injected at a rate of 100 nl/min via a microcontroller-operated electrical micropump through a 34 g beveled needle (see “Viral transduction” section). Data for the condition post-MSDB injection were acquired between 20 and 60 min after the end of the injection procedure.
For focal injections into the hippocampus, we used a blocker mixture of atropine sulfate monohydrate (7.2 mm), mecamylamine hydrochloride (10 mm, catalog no. 2843; Tocris Bioscience), and methyllycaconitine citrate (20 μm, catalog no. 1029; Tocris Bioscience) dissolved in ACSF. Because, compared with the more spatially confined MSDB, the hippocampus is a very large structure, we injected 10 × 200 nl at 100 nl/min, amounting to a total volume of 2 μl over a time course of 1 h to allow diffusion of blocker solution over the entire dorsal hippocampus. Data for the condition posthippocampal injection were acquired 10 min after the end of the injection procedure for up to 90 min.
In vivo optical stimulation.
For optical stimulation, a software-controlled 473 nm diode laser (LuxX 473-80; Omicron-Laserage Laserprodukte) was coupled via a FC/PC connection to a multimode light fiber (0.22 numerical aperture, 550 μm core, BFL22-550; Thorlabs). The laser power was adjusted before each experiment to yield a light power of 45 mW exiting the bare light fiber end.
Immunohistochemistry.
Heart perfusion for rapid brain fixation was performed as described for the reconstruction of electrode position. Formalin-fixated brains were stored until slicing in storing solution (PBS with 0.1% sodium azide; catalog no. 822335; Merck) at 4°C. Fifty-micrometer-thick coronal slices were cut with a vibratome in PBS and kept in storing solution in 24-well plates (catalog no. 83.3922; Sarstedt) at 4°C until staining. For staining, slices were briefly washed with PBS and submerged for 10 min in 0.25% Triton X-100 (Sigma-Aldrich) dissolved in PBS. For the following steps, slices were washed three times for 10 min between each solution change. Slices were submerged overnight at 4°C in PBS solution containing the first antibodies and for 2 h at room temperature in PBS solution containing the secondary antibodies. For costaining of ChAT and eYFP, goat anti-ChAT affinity-purified polyclonal antibody (catalog no. AB 144P; Merck) diluted 1:500 and rabbit anti-GFP affinity purified polyclonal antibody (catalog no. ab6556; Abcam) diluted 1:1000 were used as first antibodies and Cy3-conjugated donkey anti-goat-IgG polyclonal antibody (catalog no. AP180C; Merck) diluted 1:1000 and FITC-conjugated donkey anti-rabbit-IgG polyclonal antibody (catalog no. 711-096-152; Dianova) diluted 1:1000 were used as secondary antibodies. For costaining of PV and eYFP, rabbit anti-PV serum (catalog no. PV 25; Swant) diluted 1:1000 and goat anti-GFP polyclonal antibody (ab5449; Abcam) diluted 1:1000 were used as first antibodies and Cy3-conjugated donkey anti-rabbit-IgG polyclonal antibody (catalog no. 711-156-152; Dianova) diluted 1:1000 and FITC-conjugated donkey anti-goat IgG polyclonal antibody (catalog no. 705-095-147; Dianova) diluted 1:1000 were used as secondary antibodies. After the last washing step, slices were mounted onto microscope slides (Superfrost Plus; Thermoscientific) in Aqua-Poly/Mount (Polysciences) mounting medium covered with coverslips (Engelbrecht, Medizin- und Labortechnik).
LFP analysis.
LFP data were digitally downsampled to 1 kHz. Power spectral density analysis was performed using the MATLAB (The MathWorks) software toolbox “FieldTrip” (Oostenveld et al., 2011). Signal preprocessing involved demeaning of the signal and 50 Hz line noise removal via a Fourier notch filter (bandwidth <1 Hz).
For quantification of stimulation-induced theta activity, we calculated the corrected theta peak power as follows: power spectral density was determined for every trial for a 10 s baseline period and a 10 s period beginning and ending 2 s later than the 10 s optogenetic stimulation period to account for the delayed onset and offset of induced theta oscillations and then averaged across trials for each animal. For calculation of power spectral density, the signal was tapered with Slepian sequences and multitaper fast Fourier transform was performed with a spectral smoothing of ±0.5 Hz. Theta peak power was measured relative to the power of the adjacent frequencies. The power of the adjacent frequencies contributing to the absolute power value at the theta peak frequency was estimated by linear interpolation between the minima surrounding the theta peak. If no theta peak was detectable (as usually in the baseline period), the theta peak power was considered to be zero. The optogenetic stimulation effects were then quantified as the difference between the theta peak power during stimulation and the theta peak power during the baseline period, yielding the corrected theta peak power.
For analyzing the time course of the decrease in stimulation-induced theta oscillations by the incremental hippocampal blocker mixture injections, power spectral density was determined for the 30 s baseline period and a 10 s period beginning and ending 2 s later than the 10 s optogenetic stimulation period (see above) for each trial in every animal. z-scores were calculated for the baseline and stimulation-associated periods to reflect the change in power spectral density in units of the SD of baseline power spectral density across trials. Baseline corrected z-scores reflect the difference between z-scores of the stimulation-associated period and the z-scores of the baseline period.
To reflect changes in the broader low gamma range reliably, we quantified low gamma power within the frequency range from 26–48 Hz for 10 s baseline and stimulation epochs. Power spectral density plots often showed sharp peaks at exactly the stimulation frequency and its higher harmonics. Because we could not rule out the possibility that these peaks are artifacts of unspecific stimulation, we excluded the stimulation frequencies and their first two harmonics (±0.5 Hz) from our gamma power analysis. Optogenetic stimulation effects were calculated as the difference between the gamma power during the stimulation period and the baseline period. To assess the effect size of systemic atropine application on changes in corrected theta peak power or corrected low gamma power, we compared the area under the curve over stimulation frequencies from 3–40 Hz preapplication versus postapplication of systemic atropine and tested for statistical significance via a Wilcoxon signed-rank test or Student's paired t test.
To analyze the power change over time, time-frequency analysis using Hanning taper was performed with a 5 s sliding time window moving over the data in 0.625 s steps. A z-score was assigned to each time bin and frequency bin for each single trial using the full epoch trial length as the “baseline” for z-score calculation. z-scores were then averaged across trials and classical prestimulus baseline corrections were performed to make the prestimulus z-score values oscillate around zero. This approach has been shown to be more robust against single trial noise than classical correction methods (Grandchamp and Delorme, 2011).
For quantification of LFP power changes at the stimulation frequencies during stimulation of PV+ MSDB neurons, z-scores were averaged across the 5 s midtime interval of stimulation and across ±0.2 Hz around the stimulation frequency.
Single unit analysis.
For offline spike sorting of unit activity, the broadband signal was digitally high-pass filtered (0.3–3 kHz, second-order elliptic filter with 0.1 dB of ripple in the pass band and a stop band 40 dB down from the peak value in the pass band). Unsupervised automatic spike detection and sorting, followed by manual adjustment of the clusters, was performed using the MATLAB (The MathWorks) software toolbox “Wave_clus” (Quiroga et al., 2004). The threshold for spike detection was set to σ = median
z-scores reflecting the change of spiking rate relative to baseline were calculated for time bins of 5 s by subtracting the mean firing rate of the prestimulus baseline (i.e., the first 30 s of recording) from the trial-averaged firing rates at each time bin and dividing these values by the SD calculated across all time bins of all trials. If the basal spiking rate was zero in each time bin of every trial but positive during stimulation periods (indicating a very strong modulation effect), the z-score during stimulation would be infinite due to a SD of zero during baseline. To include these units into the analysis, an SD was estimated on the assumption that there was one spike during the entire baseline period.
For the quantification of the optogenetic stimulation effect on each unit's firing rate, the z-scores of the time bins during stimulation (30–40 s and 70–80 s) were averaged. At the single unit level, each cell responded either with a positive or a negative change of firing rate upon stimulation. To quantify the modulation effect at the population level, we calculated a modulation index as the absolute value of the area hyperbolic sine (arsinh) of the firing rate z-scores during stimulation. Taking the arsinh of the z-scores takes into account that the z-score distribution resembles a lognormal distribution rather than a normal one. In contrast to a logarithmic scale, the arsinh is defined for both positive and negative values. Taking the absolute value makes the modulation index insensitive to the sign of the modulation; that is, a unit with increased spiking during stimulation is evaluated as equally modulated as a unit with decreased spiking during stimulation. Note that, at the population level, an increase of modulation would manifest itself in increasing the positive z-scores but decreasing the negative z-scores, whereas a decrease in modulation would result in shifting both positive and negative z-scores to zero. To quantify the effect of blocker injection compared with ACSF control injections, the difference between the modulation index before and after injection was calculated for each unit and termed the delta modulation index.
Spike-phase coupling analysis.
The LFP signal was recorded from an electrode located inside or near the principal cell layer, but from which no units were extracted to prevent contribution of the spike signal itself to the phase of the LFP signal. For offline spike-phase coupling analysis, the LFP signal was downsampled to 2 kHz and the mean of the signal was subtracted from each data point (demeaning) to make the signal oscillate around zero. After band-pass filtering in the theta range of 3–6 Hz with a second-order Butterworth filter, the left and right tails of the signal, each containing 1% of the total signal length, were multiplied with the rising and falling flanks of a modified Welch window. The instantaneous phase could then be determined via a Hilbert transformation so that each spike could be assigned its instantaneous LFP theta phase. To quantify changes in spike-phase coupling during stimulation, spike-phase coupling was analyzed for a 30 s baseline period and the stimulation periods (pooled 10 s periods of 12 and 20 Hz stimulation). To equalize the number of spikes under these two conditions, spikes were randomly deleted from the condition that contained more spikes. All recording sites were located inside or very close to the CA3 pyramidal cell layer.
In vitro patch-clamp recordings.
Experiments in MSDB slices were performed at least 2 weeks after the virus injection. For obtaining slices, mice were deeply anesthetized with ketamine (300 mg/kg body weight; WDT) and xylazine (60 mg/kg body weight; Bayer). Brains were removed and transferred into cold sucrose-containing carbogen-saturated ACSF containing the following (in mm): NaCl, 60; sucrose, 100; KCl, 2.5; NaH2PO4, 1.25; NaHCO3, 26; CaCl2, 1; MgCl2, 5; and d-glucose, 20; Sigma-Aldrich). Horizontal or coronal slices of the MSDB (300 μm) were cut on a vibratome (Leica VT 1200 S), incubated for 30 min at 37°C, and transferred into ASCF containing the following (in mm): NaCl, 125; KCl, 3; NaH2PO4, 1.25; NaHCO3, 26; CaCl2, 2.6; MgCl2, 1.3; and d-glucose, 15; Sigma-Aldrich). For electrophysiology, slices were transferred into a submerged chamber and superfused with carbogen-saturated ACSF (speed of superfusion: 3 ml/min at 35°C). Expression of ChR2-eYFP in MSDB neurons was verified using an upright fluorescence microscope (Nikon Eclipse FN1) with the following filter settings (in nm): excitation: 500/24; dichroic: 520; emission: 542/27. Whole-cell patch-clamp recordings were then obtained from identified fluorescent cells or nonfluorescent cells with the help of a fluorescence microscope (Nikon Eclipse FN1) and using infrared differential interference contrast microscopy. Pipettes were made using a horizontal puller (Model P-97; Sutter Instruments) and borosilicate glass capillaries (GB150F-8P; Science Products).
Electrode resistance in the bath ranged from 3 to 5 MΩ. The intracellular solution for whole-cell current-clamp recordings contained the following (in mm): K-gluconate, 140; 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid (HEPES-acid), 5; ethylene glycol tetraacetic acid (EGTA), 0.16; MgCl2, 0.5; sodium phosphocreatine, 5; and 0.3% biocytin. Voltage- and current-clamp experiments were performed with a Multiclamp 700B amplifier (Molecular Devices). Data were sampled at 10–50 kHz with a Digidata 1322A interface (Molecular Devices) controlled by pClamp Software (Molecular Devices) and stored on a hard disk for offline analysis.
In those experiments in which cholinergic axons were stimulated while recording from septal neurons, the neurons were classified based on the properties of genetically identified ChAT+ or PV+ neurons (Table 1). Classification was performed by H.B., who was blinded to the results of the optogenetic stimulations. As a parameter for segregating septal cell populations, the action potential half-width was used, with cells having narrow action potentials (<0.7 mV) classified as putative PV+ neurons. These cells also had large fast afterhyperpolarizations (fAHPs) compared with the putative ChAT+ population (−9.4 ± 1.7 vs −3.6 ± 1.6 mV, mean ± SEM, p = 0.027, t test), consistent with the properties of the genetically identified populations (Table 1). Action potential properties were analyzed as follows. Action potential threshold was determined as the voltage where the first derivative of the voltage trace exceeded 8 mV/ms. The half-width was determined as the action potential width at an amplitude 50% between the threshold and peak. The fAHP amplitude was determined as the difference between the threshold and the maximal repolarization observed during the first 20 ms after the action potential onset. For all measurements, action potentials were selected that occurred within the first 50 ms after onset of the current injection. In all cells, the lowest possible current injections displaying such action potentials were selected.
In vitro optogenetic stimulation.
Light stimulation of individual neurons in the MSDB (coronal slices) was performed via the microscope objective (Nikon NIR Apo 60×) using a galvanometer-based scanning system (UGA-40, DL-473; Rapp Optoelectronics) coupled to a 473 nm diode-pumped solid state laser (DL-473; Rapp Optoelectronics). eYFP-expressing neurons in the medial septum were targeted with 10 s trains of brief flashes of light (20 ms up to 2 mW laser power) that caused clear light-evoked responses in patch-clamp recordings. Stimulation frequencies ranged from 5 to 40 Hz. To assess the effects of stimulation of ChR2+ cholinergic neurons on other types of septal neurons, we used 5 s stimulus trains at a power of up to 60 mW using a 473 nm diode laser (LuxX 473-80; Omicron-Laserage Laserprodukte) coupled into a customized multimode light fiber (0.22 numerical aperture, 550 μm core, BFL22-550; Thorlabs) and 40 μm 4-aminopyridine (4-AP; Tocris Bioscience) was added to the ACSF for reliable optical stimulation. Additional recordings with longer 10 s stimulus trains were performed in the absence of 4-AP. In these experiments, neurons were classified based on the properties of genetically identified ChAT+ or PV+ neurons (Table 1). Classification was done by H.B., who was blinded to the results of the optogenetic stimulations. The end of the optical fiber was placed immediately above the brain slice surface to illuminate the MSDB. Optogenetically induced membrane depolarizations were measured relative to baseline.
Reporting of ANOVA.
One-way and two-way ANOVA results are reported according to standard criteria as follows: With dfbetween and Vbetween as degrees of freedom and variance between the conditions of the tested factor, respectively, and dfwithin and Vwithin as degrees of freedom and variance within conditions, respectively. Interaction between two factors is reported in a like manner.
Results
In vivo optogenetic activation of cholinergic MSDB neurons induces hippocampal rhythmogenesis
To achieve light-based stimulation of cholinergic MSDB neurons, we used knock-in mice expressing Cre recombinase under the control of the choline acetyltransferase promoter (ChAT-IRES-Cre; Fig. 1A and Materials and Methods). These mice were stereotactically injected with an rAAV that allows Cre-dependent expression of channelrhodopsin 2 (ChR2-H134R) fused to the eYFP. Robust ChR2-eYFP expression could be observed in cholinergic neurons (43%, n = 15 slices from 5 mice; Fig. 1A), with 84% of the ChR2-eYFP neurons showing clear ChAT immunoreactivity. We obtained patch-clamp recordings from cholinergic MSDB neurons, which showed characteristic slow-firing properties, as described previously (Griffith and Matthews, 1986; Markram and Segal, 1990; Gorelova and Reiner, 1996; Serafin et al., 1996; Sotty et al., 2003). Light-based stimulation at 473 nm with a laser focused onto the neuronal somata reliably elicited action potentials, even with long-duration stimulus trains, in all cells (10 s, spiking reliability quantified as probability to elicit action potentials per light stimulus of 1 for frequencies up to 5 Hz and reliabilities of 0.88 ± 0.35, 0.58 ± 0.46, and 0.12 ± 0.25 for 12, 20, and 30 Hz, respectively, mean ± SD of n = 8 cells; Fig. 1B).
After establishing light-based stimulation of cholinergic MSDB neurons, we turned to in vivo recordings to assess the effects of cholinergic activation on hippocampal rhythmogenesis. We first recorded LFPs from up to 32 channels of a four-shank silicon probe spanning several layers of the dorsal hippocampus (Fig. 1C). Optogenetic stimulation of ChR2+ cholinergic MSDB neurons via a light fiber implanted just above the MSDB at different stimulation frequencies caused marked changes in hippocampal rhythmicity (see Fig. 1C, right, for example recording). Most notably, virtually all recordings displayed an increase in theta and low gamma power, which often persisted for several seconds after cessation of stimulation. This effect was observed in all hippocampal subfields, as exemplified by power spectra and time-frequency plots of power spectral density [Fig. 1D,E, respectively, examples of CA1, CA3, and dentate gyrus (DG) LFP recordings, data from 11 mice with 3–6 trials per mouse]. The most robust effects were observed in the theta range (Fig. 1D,E, insets). Notably, increases in synchronization occurred in a narrow frequency range, with a suppression of adjacent frequencies (Fig. 1D, insets). We systematically varied the frequency with which light-based MSDB stimulation was performed (3–40 Hz). The frequency of peak theta synchronization was significantly correlated with the frequency of MSDB stimulation (Fig. 1F, r = 0.88 for CA1, r = 0.97 for CA3, and r = 0.96 for DG, p < 0.001, r = Pearson's correlation coefficient, n = 6 mice, 4–6 trials per mouse). Likewise, the baseline corrected theta peak power was correlated with stimulation frequency (Fig. 1G, r = 0.68 for CA1, r = 0.92 for CA3, and r = 0.89 for DG, p < 0.05 for CA1, and p < 0.001 for CA3 and DG, n = 6 mice, 4–6 trials per mouse). In addition to the correlation analyses, two-way ANOVA with hippocampal subfield as one factor and stimulation frequency as the other factor revealed a significant effect of stimulation frequency on theta peak frequency (FStimulation frequency(9,149) = 18.88, p < 0.0001, FSubfield(2,149) = 1.54, p = 0.217, FStimulation frequency*Subfield(18,149) = 0.45, p = 0.974), and significant effects of both subfield and stimulation frequency on theta peak power (FSubfield(2,150) = 30.39, p < 0.0001, FStimulation frequency(9,150) = 1.98, p < 0.05, FStimulation frequency*Subfield(18,150) = 0.15, p > 0.99). However, it should be noted that the magnitude of both effects was not very large, with a change of theta peak frequency from 3.8–4.6 Hz over the whole range of stimulus frequencies.
Similarly, gamma power was correlated with stimulation frequency in hippocampal subfields CA1, CA3 and DG (Fig. 1H, r = 0.72 for CA1, r = 0.85 for CA3, and r = 0.87 for DG, p < 0.05 for CA1, and p < 0.01 for CA3 and DG, n = 6 mice, 4–6 trials per mouse). In addition, statistical analysis using two-way ANOVA with hippocampal subfield as one factor and stimulation frequency as the other factor revealed a significant impact of the hippocampal subfield and the stimulation frequency on gamma power (FSubfield(2,150) = 5.05, p < 0.01, FStimulation frequency(9,150) = 3.32, p < 0.001, FStimulation frequency*Subfield(18,150) = 0.55, p = 0.927). As expected, systemic application of atropine, a competitive antagonist of the muscarinic acetylcholine receptor (50 mg/kg body weight), completely abolished the induction of theta rhythmic activity (Fig. 1G, p = 0.031, Wilcoxon signed-rank test, n = 6 mice with one value missing for CA1 at 40 Hz stimulation, 3–6 trials per preatropine and postatropine condition and mouse, respectively). Stimulation-induced increase in low gamma activity was not significantly changed in regions CA1, CA3, or DG (Fig. 1H, p = 0.054, p = 0.220, and p = 0.241, respectively, paired t test, n = 6 mice, 3–6 trials per preatropine and postatropine condition and mouse, respectively).
Interneuron and principal cell firing is differentially modulated by cholinergic MSDB neurons
To assess how activation of cholinergic MSDB neurons affects the activity of hippocampal neurons in vivo, we identified spikes from the high-pass-filtered LFP signal and clustered the spikes into single units (see Materials and Methods). Within the CA3 region, we discriminated putative interneurons and principal cells on the basis of their waveform and autocorrelogram according to previously published criteria (Fig. 2A,B; Csicsvari et al., 1998). Using this classification, most of the recorded units could be clearly assigned (Fig. 2B; 582/671 neurons from 42 mice, 197 putative interneurons from 36 mice, 385 putative principal cells from 39 mice, 3–10 trials per mouse). Most interneurons responded to the stimulation with an increased spiking rate, whereas the majority of principal neurons showed decreased spiking rates (Fig. 2C for examples; Fig. 2D). Accordingly, the mean normalized spiking rate was significantly increased for putative interneurons, but decreased for putative principal cells during stimulation (Fig. 2E, χ2(23,4704) = 128.2, p < 0.0001, and χ2(23,9216) = 990.3, p < 0.0001, respectively, Kruskal-Wallis test for difference between 0.5 s time bins; * indicates significant difference between one time interval against each of the baseline time intervals, p < 0.05, Tukey–Kramer post hoc test). In a subset of these recordings, we applied systemic atropine (see Materials and Methods). This allowed us to determine atropine effects on light-evoked responses in 16 putative interneurons and 35 putative principal neurons. Systemic atropine application diminished cholinergic modulation of putative interneurons, whereas the modulation of putative principal cells was not significantly altered (Fig. 2F,G; * indicates significant difference between modulation indices, p < 0.05, Wilcoxon signed-rank test, n = 16 putative interneurons from six mice, and n = 35 putative principal cells from five mice, 3–6 trials per preatropine and postatropine condition and mouse, respectively).
Stimulation-induced hippocampal theta requires an intraseptal relay
Cholinergic MSDB neurons give rise to septo-hippocampal projection fibers as well as intraseptal connections to GABAergic and glutamatergic MSDB neurons. Both of these neuron types also provide projections to the cortex and hippocampus. Therefore, it is conceivable that some effects of activating cholinergic MSDB neurons might be mediated via an intraseptal relay. We assessed the relevance of such an indirect pathway for theta synchronization. We injected atropine (300 nl, 7.2 mm, see Materials and Methods) focally into the MSDB while optogenetically stimulating cholinergic MSDB neurons (Fig. 3A, bottom). We used atropine because muscarinic ACh receptors play a major role in regulating septo-hippocampal GABAergic neurons (Alreja et al., 2000). Control animals were injected with ACSF (Fig. 3A, top). Atropine, but not ACSF injection into the MSDB, caused a complete block of optogenetically induced hippocampal theta oscillations [Fig. 3B,C; * indicates significant difference between preapplication and postapplication conditions, p < 0.05, paired t test, § indicates significant differences between ACSF (n = 6 mice) and atropine groups (n = 5 mice), p < 0.05, t test]. These results indicate that an intraseptal relay is mandatory for the generation of cholinergic theta oscillations in the hippocampus. But is synaptic acetylcholine release by MSDB projections to the hippocampus also important for hippocampal theta generation? We focally injected a blocker mixture of nicotinic and muscarinic acetylcholine receptor antagonists [mecamylamine (Mec), 10 mm, methyllycaconitine (MLA), 20 μm, and atropine, 7.2 mm, see Materials and Methods) into the dorsal hippocampus close to the recording site (see Fig. 3D for example experiments with ACh receptor blockers and ACSF injection). We chose to block both muscarinic and nicotinic ACh receptors because, in the hippocampus, most interneurons show strong excitation via nicotinic ACh receptors (Ji and Dani, 2000). In most experiments, theta induction was strongly inhibited after blocker, but not after ACSF injection [Fig. 3E,F; * indicates significant difference between preapplication and postapplication conditions, p < 0.05, paired t test, § indicates significant differences between ACSF (n = 3 mice) and Atr-Mec-MLA group (n = 5 mice), p < 0.05, t test]. After the start of the injection series for Atr-Mec-MLA, but not for ACSF, average stimulation-evoked theta power shows an incremental reduction (Fig. 3G,H; time to 50% of the effect obtained with exponential fitting 26.1 min after beginning the first injection, 20 Hz stimulation). This is consistent with a local effect of these blockers, although we cannot exclude that blockers may spread to more distant brain regions at later stages.
Our findings demonstrate that both hippocampal and septal ACh is required for proper induction of theta oscillations. In particular, the requirement for intraseptal ACh suggests that intraseptal connectivity is essential for mediating hippocampal theta induction. We therefore examined the effects of cholinergic neuron activation on other types of septal neurons. We first characterized genetically identified ChAT+ and PV+ GABAergic neurons in the slice preparation (see Materials and Methods) and characterized their functional properties (Fig. 4A,B). PV+ neurons were characterized by narrow action potentials with a fast upstroke and prominent fAHPs. These characteristics set them apart from ChAT+ neurons (Table 1). Subsequently, we activated cholinergic neurons optogenetically in septal slices and recorded from non-ChR2-expressing medial septal neurons. Non-ChR2-expressing neurons were classified into putative PV+ and other neurons based on their functional properties. Whereas a single light stimulation pulse elicited only small effects in non-PV+ neurons, it caused a slow depolarization in putative PV+ neurons (Fig. 4C, top and bottom traces, respectively, Fig. 4E, quantification of average amplitude and area under the curve within 5 s after stimulation in Fig. 4G; */** indicate significant difference, *p < 0.05, **p < 0.01, t test, n = 9 and 19 for PV+ and non-PV+ neurons, respectively). Trains of stimulations reliably elicited longer-lasting slow depolarizations in both neuron types (Fig. 4D,F) that were significantly larger in putative PV+ neurons (Fig. 4H; * indicates significant difference, *p < 0.05, t test, n = 10 and n = 16 for PV+ and non-PV+ neurons, respectively). We additionally recorded from five putative PV+ neurons using 10 s stimulation trains, an identical duration as used for the in vivo experiments. We observed a depolarization in four of five neurons. Notably, this depolarization lasted over the full 10 s time interval of the stimulus train (Fig. 4I; only the four cells showing a depolarization are shown). Of the 15 putative PV+ neurons, seven were depolarized sufficiently to generate action potentials during light-stimulation, with the time at which action potentials occurred being very variable.
These results suggest that PV+ septal neurons may be recruited by cholinergic activation and play a role in driving hippocampal theta rhythms. Indeed, PV+ MSDB neurons selectively innervate hippocampal interneurons and have long been suggested to be important for hippocampal theta rhythmicity via disinhibition of principal cells (Freund and Antal, 1988; Serafin et al., 1996; Tóth et al., 1997; Hangya et al., 2009). After expression of ChR2 in PV+ septal neurons using rAAV-mediated gene transfer (Fig. 5A), brief light pulses resulted in reliable stimulation of these neurons, even during long stimulation trains of 10 s (spiking reliability per stimulus pulse of 1 for frequencies up to 20 Hz, and reliabilities of 0.92 ± 0.09 and 0.45 ± 0.43 for 30 and 40 Hz, respectively, mean ± SD of n = 4 cells; Fig. 5B). We performed in vivo light stimulation of PV+ neurons in the MSDB and simultaneously recorded with a silicon probe in the hippocampus (n = 5 mice). Optogenetic stimulation of PV+ MSDB neurons caused a recruitment of hippocampal rhythmicity at precisely the stimulation frequency (Fig. 5C–E), unlike for the stimulation of ChAT+ MSDB neurons or light stimulation in untransduced wild-type mice (Fig. 5G,H). Remarkably, the spectral power of the oscillatory activity showed a clear frequency dependence (Kruskal–Wallis test, χ2(9,40) = 36.6, p < 0.0001 for CA1, χ2(9,40) = 21.6, p < 0.05 for CA3, and χ2(9,40) = 33.6, p < 0.001 for DG). There was a maximum within all subregions at ∼10 Hz stimulation frequency, indicating a preferred frequency of the MSDB-hippocampal network oscillation (Fig. 5F). The distinct nature of the effects of stimulating PV+ MSDB neurons can be clearly appreciated, as well as the lack of any effect in wild-type animals.
Modulation of hippocampal neuronal activity by cholinergic MSDB neurons is mediated by direct septo-hippocampal projections
We next assessed how relevant direct versus indirect MSDB projections to the hippocampus are for the observed inhibition of principal neuron activity (Fig. 2). We measured how optogenetic stimulation of ChAT+ MSDB neurons modulates the firing rate of hippocampal neurons in animals that received either focal injections of atropine into the MSDB or injections of a cholinergic blocker mixture (Fig. 3) into the hippocampus. As before, ACSF-injected animals were used as controls.
To quantify the effect on population spiking rate, we calculated a modulation index (see Materials and Methods) of single unit spiking rate modulation for each unit (Fig. 6A,B). This allows quantifying the effect of ACSF control or blocker injection at the population level via calculation of the delta modulation index; that is, the difference between the modulation indices before and after injection for each cell (Fig. 6C,D). Therefore, at the population level, a mean delta modulation index of zero means no change in spiking rate modulation, whereas a negative mean delta modulation index indicates a decrease of spiking rate modulation.
Two-way ANOVA was performed on the delta modulation indices with the injection site (MSDB vs hippocampus) as one factor and the drug (ACSF vs blocker) as the other factor (Fig. 6C,D). We found a significant main effect of both site and drug for both 12 and 20 Hz stimulation conditions for putative interneurons (FSite(1,165) = 21.20, p < 0.0001, FDrug(1,165) = 13.40, p = 0.0003 for 12 Hz stimulation; FSite(1,165) = 17.03, p = 0.0001, FDrug(1,165) = 17.96, p < 0.0001 for 20 Hz stimulation) as well as principal cells (FSite(1,300) = 6.50, p = 0.0113, FDrug(1,300) = 8.85, p = 0.0032 for 12 Hz stimulation; FSite(1,300) = 17.46, p < 0.0001, FDrug(1,300) = 13.81, p = 0.0002 for 20 Hz stimulation). There was a significant interaction between site and drug for interneurons under both stimulation conditions (FSite*Drug(1,165) = 15.84, p = 0.0001 and FSite*Drug(1,165) = 11.70, p = 0.0008 for 12 and 20 Hz stimulation, respectively) and for principal cells for the 12 Hz stimulation condition only (FSite*Drug(1,300) = 6.62, p = 0.0106 and FSite*Drug(1,300) = 0.44, p = 0.5081 for 12 and 20 Hz stimulation conditions, respectively). Whereas focal atropine injection into the MSDB had no effects on single unit modulation (p > 0.05, Tukey–Kramer post hoc test), focal injection of a mixture of atropine, Mec, and MLA into the hippocampus abolished spiking rate modulation (p < 0.05, Tukey–Kramer post hoc test) of putative interneurons for both stimulation conditions (Fig. 6C) and strongly reduced spiking rate modulation of putative principal cells, again under both stimulation conditions (Fig. 6D). The onset of the effects of blocker injections into the hippocampus was plotted by quantifying the modulation index in 6 min bins and showed a clear onset of the effect within 10 min of drug application (Fig. 6E,F; time to reach 50% of the effect obtained with exponential fitting for interneurons 14.1 min after beginning the first injection; for principal neurons 11.7 min after beginning the first injection, 20 Hz stimulation). These results suggest that, in contrast to theta generation, modulation of hippocampal unit activity by cholinergic MSDB neurons requires direct septo-hippocampal projections, not a septal relay.
We have also determined the effects of blocker injections on basal discharge rates. Injection of cholinergic blockers into the MSDB did not affect basal firing rates of interneurons or pyramidal neurons (Fig. 6G), but hippocampal injections reduced interneuron firing and increased pyramidal cell firing significantly (Fig. 6H).
Cholinergic stimulation increases coupling of hippocampal neuronal firing to theta phase
So far, these results show that cholinergic septal neurons induce theta synchronization, but at the same time also cause a reduction in principal neuron firing via direct septo-hippocampal projections. We considered the purpose of this dual effect and hypothesized that increasing rhythmic synaptic inputs while simultaneously hyperpolarizing the target population would lead to a more constrained action potential output that is more strictly related to the phase of ongoing theta activity (see Fig. 7 for schematic diagram). We tested this hypothesis by first examining interneuron and principal cell firing with respect to theta phase coupling (Fig. 8A,D). We used Kuiper's test to identify units with significant phase coupling (α = 0.05) during baseline and stimulation periods (p-values indicated for a representative interneuron and pyramidal cell in Fig. 8A,D, respectively). The number of both principal cells and interneurons with significant theta phase coupling increased during stimulation (Fig. 8B,E). To further analyze phase coupling at the population level, we determined the length of the mean resultant vector for each unit. This measure also revealed significantly increased phase coupling both for interneurons (Fig. 8C; p < 0.001, n = 120 from 22 mice, Wilcoxon signed-rank test) and principal cells (Fig. 8F, p < 0.01, n = 176 from 24 mice, Wilcoxon signed-rank test). When considering the phase of the mean resultant vectors only for the phase-coupled units, a preferential phase coupling was observed for interneurons around the descending phase of theta (77 ± 56°, mean ± SD; Fig. 8G) and for principal cells around the theta trough (156 ± 59°, mean ± SD; Fig. 8H).
Discussion
Our findings demonstrate that ACh release from MSDB neurons has two anatomically and functionally separable effects that act synergistically to make pyramidal neuron firing more precisely coupled to the theta oscillatory phase. First, MSDB cholinergic neurons mediate a sustained increase in hippocampal theta oscillations via an intraseptal relay. Second, direct cholinergic projections from the MSDB to the hippocampus reduce the firing of principal neurons, whereas interneurons are activated.
Our first finding was that optogenetic stimulation of MSDB cholinergic neurons induces hippocampal theta oscillations with a relatively delayed onset. In addition, we found that changing the frequency of cholinergic stimulation led to only small changes in theta frequency (∼1 Hz for a >10-fold change in stimulation frequency). Both findings are not surprising for effects mediated by metabotropic receptors via a slow second-messenger cascade. Similar effects have been observed recently in anesthetized mice (Vandecasteele et al., 2014). In freely moving mice, increases in theta power were less pronounced, likely due to a higher ACh tone in foraging or ambulatory animals, and seemed to be more related to a suppression of adjacent frequency bands (Vandecasteele et al., 2014). A consistent finding in our experiments was the suppression of frequency bands adjacent to the theta peak. Notably, slow oscillations between 1 and 3 Hz were suppressed, similar to results obtained in visual cortex during stimulation of basal forebrain cholinergic neurons (Pinto et al., 2013).
A second finding of this study was that CA3 principal neuron activity is strongly inhibited by activation of MSDB cholinergic neurons, whereas interneurons are activated. This finding is in good agreement with the recent description of a reduction in CA3 sharp wave ripple oscillations by optogenetic stimulation of MSDB cholinergic neurons (Vandecasteele et al., 2014).
We next examined the neuronal circuits underlying these two effects: theta induction and inhibition of CA3 pyramidal firing. We found that blocking MSDB muscarinic ACh receptors abolishes optogenetically induced hippocampal theta oscillations, indicating the necessity of a septal relay for theta induction. Indeed, in vitro experiments showed that cholinergic activation causes long-lasting depolarization of putative PV+ neurons, in agreement with anatomical data showing that noncholinergic MSDB neurons are contacted by putative cholinergic terminals (Bialowas and Frotscher, 1987; Leranth and Frotscher, 1989). Moreover, we demonstrate that PV+ MSDB neurons are capable of precise synchronization of hippocampal networks. PV+ MSDB neurons selectively innervate hippocampal interneurons and have long been suggested to be important for hippocampal theta rhythmicity via disinhibition of principal cells (Freund and Antal, 1988; Serafin et al., 1996; Tóth et al., 1997; Hangya et al., 2009; Wulff et al., 2009).
Cumulatively, these data suggest that cholinergic MSDB neurons recruit PV+ and perhaps other neurons within the MSDB, which then mediate hippocampal theta synchronization. This is consistent with the finding that PV+ neurons in the MSDB pace hippocampal theta oscillations (Varga et al., 2008; Hangya et al., 2009; Huh et al., 2010). These results are also consistent with the inhibition of theta oscillations by focal atropine injection into the medial septum (Kramis et al., 1975). Conversely, activating MSDB neurons by intraseptal infusion of muscarinic agonists in behaving rats causes continuous theta field activity, confirming that intraseptal cholinergic stimulation is not only necessary, but also sufficient for the induction of hippocampal theta oscillations (Lawson and Bland, 1993). Importantly, hippocampal application of cholinergic agonists in vitro is also capable of eliciting theta-like oscillations (Konopacki et al., 1987; Kowalczyk et al., 2013). It is thus important to note that hippocampal networks must also have an autonomous capability to generate theta-like activity without the medial septum. However, theta pacing by the medial septum requires an intraseptal relay.
Importantly, the inhibition of principal cells and the recruitment of interneurons were unaffected by cholinergic antagonists injected into the MSDB, indicating that they do not require a septal relay. Therefore, anatomically separable pathways are responsible for both inducing theta oscillations and reducing firing rates of CA3 neurons. The specific interneuron types that mediate cholinergic inhibition in the CA3 region can currently not be further pinpointed on the basis of single unit recordings. In principle, different types of hippocampal interneurons appear to be recruited by ACh release from cholinergic axons, both in vitro (Lawrence et al., 2006; Widmer et al., 2006; Cea-del Rio et al., 2010; Nagode et al., 2011, 2014) and in vivo (Lovett-Barron et al., 2014).
What could the functional purpose be for implementing these two separable effects in CA3 pyramidal neurons? The inhibition of CA3 firing, mediated by the direct cholinergic septo-hippocampal pathway, confirms a prediction made by an influential model for hippocampal encoding and retrieval (Hasselmo et al., 2002). In this model, hippocampal ACh promotes encoding in a time frame of seconds by inhibiting the CA3 autoassociative network. Both our results and the inhibition of CA3 sharp wave-ripples support this idea.
In addition, we found a significantly stronger coupling of CA3 pyramidal cell firing to theta phase during optogenetic stimulation of cholinergic MSDB neurons. This is very likely due largely to the strong enhancement in theta oscillatory activity. Nevertheless, a more precise timing of CA3 neuron firing might promote plasticity in either the autoassociative CA3 network or in CA3–CA1 projections (Pavlides et al., 1988; Hölscher et al., 1997; Orr et al., 2001; Hyman et al., 2003). Such an effect has been observed in the human medial temporal lobe and is predictive of subsequent memory performance (Rutishauser et al., 2010). In monkeys, phase locking of single unit activity was observed in the cortex during working memory tasks and this is likewise predictive of memory performance (Liebe et al., 2012). It should be noted, however, that these conclusions, in particular those related to spike-phase synchronization, have to be tempered by the fact that these data were obtained in anesthetized animals, in which principal and interneuron discharge rates are modulated by the anesthetic agent. Experiments in awake animals would be required to determine how the indirect and direct pathways are recruited in behaviorally relevant situations in vivo.
In summary, we have revealed cholinergic network motifs that act synergistically to structure the firing of hippocampal neurons temporally. These circuits may be relevant for information encoding, when cholinergic tone is increased during exploratory behavior and novelty experience (Aloisi et al., 1997; Bianchi et al., 2003).
Footnotes
- Received October 28, 2014.
- Revision received April 2, 2015.
- Accepted April 5, 2015.
This work was supported by the Deutsche Forschungsgemeinschaft (DFG Grant SFB 1089 to H.B., S.S., and F.M.; DFG German-French binational program grant to H.B.), the Federal Ministry of Education and Research (BMBF Grant 01GQ0806 to S.S.), and the ERANET Neuron EpiNet (H.B.). We thank Olivia van Ray and Margit Reitze for excellent technical assistance.
The authors declare no competing financial interests.
- Correspondence should be addressed to Heinz Beck, Laboratory for Experimental Epileptology and Cognition Research, Department of Epileptology, University of Bonn Medical Center, Sigmund-Freud-Straße 25, D-53105 Bonn, Germany. heinz.beck{at}ukb.uni-bonn.de
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