Abstract
In the absence of overt cellular pathology but profound perceptual disorganization and cognitive deficits, schizophrenia is increasingly considered a disorder of neural coordination. Thus, different causal factors can similarly interrupt the dynamic function of neuronal ensembles and networks, in particular in the prefrontal cortex (PFC), leading to behavioral disorganization. The importance of establishing preclinical biomarkers for this aberrant function has prompted investigations into the nature of psychotomimetic drug effects on PFC neuronal activity. The drugs used in this context include serotonergic hallucinogens, amphetamine, and NMDA receptor antagonists. A prominent line of thinking is that these drugs create psychotomimetic states by similarly disinhibiting the activity of PFC pyramidal neurons. In the present study we did not find evidence in support of this mechanism in PFC subregions of freely moving rats. Whereas the NMDA receptor antagonist MK801 increased PFC population activity, the serotonergic hallucinogen DOI dose-dependently decreased population activity. Amphetamine did not strongly affect this measure. Despite different effects on the direction of change in activity, all three drugs caused similar net disruptions of population activity and modulated gamma oscillations. We also observed reduced correlations between spike-rate and local field potential power selectively in the gamma band suggesting that these drugs disconnect spike-discharge from PFC gamma oscillators. Gamma band oscillations support cognitive functions affected in schizophrenia. These findings provide insight into mechanisms that may lead to cortical processing deficits in schizophrenia and provide a novel electrophysiological approach for phenotypic characterization of animal models of this disease.
Introduction
Schizophrenia is associated with aberrant information processing in the prefrontal cortex (PFC) (Weinberger et al., 1986; Goldman-Rakic, 1994; Lewis, 1995; Andreasen et al., 1997; Artigas, 2010). The mechanism underlying this disruption is poorly understood. Psychotomimetic drugs are an important modeling tool in this regard because, despite acting on distinct groups of receptors, they similarly disrupt behavior. For example, serotonin (5HT)2A agonists produce hallucinations and sensory disturbances in humans, and hyperlocomotion and cognitive deficits in rodents (Bowers and Freedman, 1966; Vollenweider et al., 1998; Aghajanian and Marek, 2000; González-Maeso et al., 2007; Geyer and Vollenweider, 2008). Likewise, NMDA receptor antagonists and amphetamine produce schizophrenia-like symptoms in humans and aberrant locomotion and cognition in rodents (Snyder, 1976; Krystal et al., 1994). A prominent theory in the field is that, although these drugs act on different receptor and neurotransmitter systems, they all disrupt PFC information processing by disinhibiting pyramidal cells (Aghajanian and Marek, 2000; Lewis and Moghaddam, 2006; Gray and Roth, 2007a,b; González-Maeso et al., 2008; González-Maeso and Sealfon, 2009).
Application of 5HT2 agonists (and serotonin) to medial PFC slices produces excitatory postsynaptic effects (Aghajanian and Marek, 1997; Marek and Aghajanian, 1999; Zhang and Marek, 2008) and increases discharge of medial PFC neurons projecting to midbrain areas in anesthetized animals (Puig et al., 2003). Likewise, NMDA antagonists increase the activity of PFC neurons (Jackson et al., 2004; Homayoun and Moghaddam, 2008). These findings have had important mechanistic implications for schizophrenia and drug target development (Marek and Aghajanian, 1998a; Moghaddam, 2003, 2004; Gray and Roth, 2007a; González-Maeso et al., 2008; González-Maeso and Sealfon, 2009). However, despite evidence of an excitatory role for serotonergic hallucinogens, they inhibit neurons in motor, orbitofrontal (OFC), and anterior cingulate (ACC) cortices of anesthetized animals (Ashby et al., 1989; El Mansari and Blier, 2005). More importantly, their impact on PFC discharge or local field potential (LFP) oscillations in awake animals is unknown. This is critical as the excitatory influence of NMDA receptor antagonists on PFC neurons is observed selectively in awake animals (Jackson et al., 2004; Homayoun and Moghaddam, 2007) but not slice preparations (Wong et al., 1986; Huettner and Bean, 1988).
Here, we compared the effects of a serotonergic hallucinogen with other psychotomimetic drugs on PFC neuronal activity of freely moving rats, to determine whether they share a common cellular or network outcome. We measured neuronal activity in OFC and ACC, two regions implicated in the pathophysiology of schizophrenia (Heckers et al., 1998; Kopp and Rist, 1999; Carter et al., 2001; Alain et al., 2002; Weiss et al., 2003; Ragland et al., 2004). Animals were implanted with stationary electrode arrays and received the hallucinogenic 5HT2A/C agonist 1-(2,5-dimethoxy-4-iodophenyl-2-aminopropane) (DOI), NMDA antagonist MK801, and amphetamine in a randomized design. We analyzed neuronal population activity, LFP power, and correlations between spike-discharge and LFP power. We find differential modulation of population activity but similarly reduced network integrity and decoupling of spiking and gamma power. These convergent outcomes are mechanisms by which diverse molecular factors may disrupt cortical function.
Materials and Methods
Subjects and surgical procedure.
Male Sprague Dawley rats (∼400 g, Harlan) were housed on a 12 h light/dark cycle (lights on at 7:00 P.M.). Microelectrode arrays were implanted bilaterally in the OFC (n = 11 rats) or in the OFC and contralateral ACC (n = 6 rats) of isoflurane anesthetized rats, and secured with dental cement for chronic recording, as previously reported (Jackson et al., 2004). The following coordinates (Paxinos and Watson, 1998) were used (relative to bregma): ACC = +3.0 mm anterior, +0.5 mm lateral, − 2.2 mm ventral from skull; OFC = +3.0 mm anterior, +3.3 mm lateral, − 4.5 mm ventral. Recording sessions began after 7 d of postoperative recovery. At the completion of all recordings, rats were anesthetized with 400 mg/kg i.p. chloral hydrate and perfused with saline and 10% buffered formalin. Coronal slices of frontal cortex were taken from each brain and cresyl-violet stained. Locations of electrode arrays were confirmed via light microscope. Data from rats with incorrect placements were discarded from all analyses. All procedures were in accordance with the National Institute of Health's Guide to the Care and Use of Laboratory Animals, and approved by the University of Pittsburgh Institutional Animal Care and Use Committee.
Experimental design.
Neuronal activity was recorded from freely moving rats in a clear polycarbonate home cage with bedding. Rats were habituated to all aspects of the recording process for 2 d. After a 30 min baseline recording, animals received an intraperitoneal injection of DOI, amphetamine, MK801 or saline vehicle. Neuronal activity was recorded for 120 min after injection. Multiple doses of +/−DOI (1.0, 3.0, and 5.0 mg/kg) were used because this was the first electrophysiology study to examine the effects of this drug in awake PFC. Previous reports have demonstrated that similar doses of DOI produce psychotomimetic effects (Pranzatelli, 1990; Gewirtz and Marek, 2000; Zhang and Marek, 2008). The doses of MK801 (0.1 mg/kg) and amphetamine (2.0 mg/kg) were chosen based on previous studies showing a significant influence on PFC single unit activity and PFC-dependent behaviors (Aultman and Moghaddam, 2001; Homayoun et al., 2004; Jackson et al., 2004; Moghaddam and Homayoun, 2008). Each drug was administered according to a random design with a 7 d washout between injections.
Electrophysiology.
Single unit activity and LFP were recorded simultaneously via bilateral eight-channel Teflon-insulated stainless steel 50 μm microwire arrays (NB Laboratories). Unity-gain junction field effect transistor headstages were attached to a headstage cable and commutator that did not restrict the animal's movement. Signals were amplified via a multichannel amplifier (Plexon). Spikes were bandpass filtered between 220 Hz and 5.9 kHz, amplified 500×, and digitized at 40 kHz. LFP was bandpass filtered between 0.7 Hz and 8 kHz, amplified 1000×, and digitized at 40 kHz. The digitized LFP recording was down sampled to 1 kHz. Single unit activity was then digitally high-pass filtered at 300 Hz and LFP were low-pass filtered at 125 Hz. Threshold crossing spike waveforms and LFP were stored for offline analysis. Single units were sorted using standard techniques and the Offline Sorter software package (Plexon). Single unit activity was only used if the neuron displayed a stable waveform throughout the session. Because each animal was allowed 1 week of washout between recording sessions, we chose to treat units recorded in different sessions as different units despite the fact that the same unit may have been serially recorded. This approach allowed for the most conservative assessment of unit identity. All units meeting these criteria were used in all single unit analyses. We did not remove putative fast-spiking interneurons from our samples as <3% of neurons met criteria for putative fast-spiking interneurons. Furthermore, there was no correlation between baseline discharge rate and the direction of any drug effect (see Results).
Data analysis.
Analysis of single unit data was conducted with Matlab (MathWorks) and SPSS statistical software (IBM). The first 3 min of the 30 min baseline were excluded to ensure a stationary baseline. The last 12 min of the postinjection period were excluded to yield a postinjection period four times longer than the 27 min baseline period (108 min) (Fig. 1A). For all single unit analyses, 180 s bins were used.
Differences in baseline firing rate between samples of units were assessed with Kruskal–Wallis tests. Single unit activity was Z-score normalized against the mean baseline firing rate. In some analyses, normalized activity was absolute value transformed to examine the net change in activity without respect to direction of change. Changes in population activity were assessed by computing the normalized mean baseline and postinjection activity of all units, during the baseline, and two 27 min bins following the injection (27–54 and 78–105 min postinjection). These time periods were chosen because they generally contained stationary population and single unit activity levels. These periods were used for all statistical comparisons, although data from the entire experiment are displayed for clarity. Similar to previous reports, a unit was classified as significantly activated or inhibited if three or more consecutive bins exceeded a 95% confidence interval around the baseline mean (Homayoun et al., 2005; Homayoun and Moghaddam, 2007). The stringency of these criteria was verified by bootstrap analysis of the baseline activity (10,000 samples; expected false-positive rate = 0.002). These criteria for classification were chosen to be sensitive to a wide range of changes in discharge rate, although it should be noted that the majority of drug-induced changes in discharge rate were of longer duration. We assessed the cross-correlation in spike-discharge between each pair of simultaneously recorded unit pairs within each region. For this analysis, spike counts were quantified in 10 ms bins, inside a 200 ms window centered on the reference spike. A pair was classified as having a significant response if three consecutive bins of the resulting cross-correlation function exceeded a 99% confidence interval of the expectation under the assumption of a Poisson distribution.
In rats with implants in both OFC and ACC, LFP data were analyzed using customized Chronux (http://www.chronux.org) routines (Mitra and Bokil, 2008). LFP voltage traces were Fourier transformed inside of a sliding time window of 4 s, with 2 s steps. A standard multitaper approach was used (Mitra and Pesaran, 1999; McCracken and Grace, 2009) in which nine tapers were applied to each window. Power spectra were calculated from the multitapered Fourier transformations and spectral data in each frequency bin were Z-score normalized against the baseline period, and each animal's data were averaged together to yield group mean spectral data. Each animal's spectral power during the baseline and two postinjection bins (27–54 and 78–105 min postinjection) was used for statistical comparisons. To more accurately describe the modulation of power in the gamma band, we divided gamma into low (30–55 Hz) and high (55–80 Hz) gamma bands for all analyses. We assessed the relationship between gamma power and single unit discharge rate with a Pearson correlation. Each unit's discharge rate and the simultaneously recorded high and low gamma band power were correlated across nine consecutive 180 s bins. The correlation coefficient of each unit was transformed to a Fisher's Z score. Normalized correlation coefficients were averaged to yield a population mean correlation during the baseline, early postinjection, and late postinjection period. While correlations between units are often strongly associated with single unit and gamma power correlations, we did not factor between unit correlations into our calculations.
Statistical testing of LFP power and single unit population data followed the same procedure. Interactions between drug groups and time were assessed with two-way repeated-measures ANOVA for both OFC and ACC. One-way between groups ANOVA was used to detect differences between each drug group in a given time bin (baseline, early, or late postinjection). Post hoc analyses were done with protected Fisher's LSD tests. For each drug group, one-way repeated-measures ANOVA was used to determine whether postinjection time points were significantly different from baseline. For all tests, the Greenhouse–Geisser correction was applied as necessary. Statistically significant differences in baseline firing rate between samples were assessed with Kruskal–Wallis tests. Spearman rank-order correlation was used to assess the relationship between postinjection activity and baseline discharge rate. Pearson correlation was used to assess the relationship between dose of DOI and neuronal activity. For single unit data, differences in the distribution of responses (activated, inhibited, or no change) between drug and vehicle samples were assessed with a χ2 test of independence. A similar procedure was used to assess modulation of the proportion of units with a significant cross-correlation. All α levels were set to 0.05.
Results
Distinct effects of DOI, MK801, and amphetamine on unit activity of prefrontal cortex neurons
Drugs were administered in a randomized design (Fig. 1A). In total, 527 OFC and 177 ACC units were recorded from histologically verified electrodes (Fig. 1B). There was no difference in mean baseline discharge rate before administration of each drug (Table 1). There was no systematic correlation between single unit baseline firing rates and the postinjection effect in any group (Table 2). Each drug evoked sustained changes in the activity of a subpopulation of units, whereas vehicle was associated with weaker and more sporadic changes in activity (Fig. 2A–L). In OFC and ACC, a significant interaction between drug group and time was detected (OFC, F(10,1076) = 11.497; ACC, F(10,350) = 7.188; all p < 0.001). These effects were caused by significant differences between drug groups during the two postinjection bins, but not the baseline period (OFC early bin, F(5,546) = 13.507; OFC late bin, F(5,546) = 11.611; ACC early bin, F(5,180) = 8.740; ACC late bin, F(5,180) = 7.856; all p < 0.001).
In the OFC, 1.0 mg/kg DOI significantly reduced population activity compared with baseline in both postinjection bins (Fig. 3A; F(2,190) = 6.309, p = 0.008). Larger doses produced greater population suppression compared with baseline (3.0 mg/kg, F(2,156) = 17.618; 5.0 mg/kg, F(2,192) = 28.151; all p < 0.001) or vehicle (Fig. 3A). These effects on population activity were echoed by the effects of DOI on individual units. While 1.0 mg/kg DOI did not strongly affect the activity of many units, larger doses of DOI inhibited the majority of units tested and produced significant differences in the distribution of responses compared with vehicle (Fig. 3B; 3.0 mg/kg, χ2(2) = 31.240; 5.0 mg/kg, χ2(2) = 25.582, all p < 0.001). The higher doses (3.0 and 5.0 mg/kg) produced similar proportions of inhibited neurons (Fig. 3B). The effect of DOI on suppressing OFC population activity was consistent throughout the recording session (Fig. 3C), and dose was negatively correlated with the early and late postinjection effect (early, r = −0.245; late, r = −0.145).
ACC population activity was suppressed by DOI in a similar fashion. Unlike larger doses of DOI, the 1.0 mg/kg dose failed to produce a significant effect on population activity (Fig. 3D). Although 1.0 mg/kg produced activation in the majority of units with a significant response, there was no significant difference in the response distribution compared with vehicle (Fig. 3E). Larger doses of DOI reduced population activity. In the early postinjection bin, 3.0 mg/kg DOI reduced population activity compared with baseline (Fig. 3D; F(2,64) = 4.922, p = 0.010). The 5.0 mg/kg dose reduced ACC population activity at both early and late postinjection bins (Fig. 3D; F(2,72) = 16.769, p < 0.001). Suppression of activity by 3.0 or 5.0 mg/kg occurred in the majority of individual units (Fig. 3E). All doses of DOI produced a sustained effect on ACC population activity (Fig. 3F). There was a negative correlation between dose of DOI and ACC postinjection effect (early, r = −0.307; late, r = −0.334).
In contrast to the effects of DOI, MK801 increased population activity in both brain regions (OFC, F(2,180) = 16.89; ACC, F(2,46) = 10.092; all p < 0.001) during both postinjection periods (Fig. 3A,D). The most common change in activity was activation, creating significant differences in the MK801 and vehicle single unit response distributions (Fig. 3B,E; OFC, χ2(2) = 19.076, p < 0.001; ACC, χ2(2) = 7.851, p = 0.020). Amphetamine increased OFC population activity compared with vehicle only in the late postinjection bin (Fig. 3A). Amphetamine nonsignificantly suppressed ACC population activity (Fig. 3D). The lack of strong effects on either population can be explained by the fact that amphetamine simultaneously increased the activity of many single units while decreasing the activity of many others, cancelling out a population effect. In both regions, this resulted in significant differences in the distribution of responses compared with vehicle (Fig. 3B,E; OFC, χ2(2) = 15.540, p < 0.001; ACC, χ2(2) = 6.510, p = 0.039). Together, DOI mediated decreases in population activity that were distinct from those of other psychotomimetic drugs.
Similar levels of population disruption by DOI, MK801, and amphetamine
Given that each drug drove both increases and decreases in single unit activity and distinctly different patterns of population activity, we reasoned that their psychotomimetic nature may arise, in part, from the net disruption of self-organized activity levels. The normalized activity of each unit was absolute value transformed to examine disruptions of activity, without respect to the direction of the disruption (Fig. 4A–D). In OFC and ACC, a significant interaction between time and drug was detected (OFC, F(10,1082) = 5.064, p < 0.001; ACC, F(10,350) = 3.093, p = 0.001). In both regions there were significant differences between drug groups in both postinjection periods (OFC early, F(5,541) = 6. 604, p < 001; OFC late, F(5,541) = 3.562, p = 0.004; ACC early, F(5,175) = 4.567, p < 0.001; ACC late, F(5,175) = 2.610, p = 0.026).
In OFC and ACC, DOI dose-dependently elevated absolute value transformed population activity above vehicle levels (Fig. 4A–D). In OFC, 1.0 mg/kg DOI produced significant disruptions of population activity only in the early postinjection bin (Fig. 4B), while this dose did not produce significant disruptions of activity in the ACC (Fig. 4C,D). Larger doses of DOI produced greater levels of population disruption in both periods and both brain regions (Fig. 4B,D). In OFC, MK801 and amphetamine also produced increased levels of disruption compared with vehicle during both the early and late postinjection periods (Fig. 4B). A similar pattern was detected in ACC (Fig. 4D). There was little difference in the magnitude of disruption produced by each psychotomimetic drug. MK801, amphetamine, and 3.0 and 5.0 mg/kg DOI all produced equivalent levels of OFC population disruption (Fig. 4B). An identical relationship was found in ACC (Fig. 4D).
Cross-correlation analysis between each pair of simultaneously recorded units within the OFC or ACC, which is a rough measure of the functional connectivity between units, detected no consistent effect of any psychotomimetic drugs (Table 3). It should be noted that, in both regions, the lowest dose of DOI decreased the proportion of significant pairs compared with baseline (Table 3; OFC early, χ2(1) = 9.133, p = 0.003; OFC late, χ2(1) = 9.756, p = 0.002; ACC early, χ2(1) = 14.990, p < 0.001; ACC late, χ2(1) = 14.990, p < 0.001). However, this should be interpreted cautiously as the vehicle sessions were characterized by instability in the proportion of pairs that possessed a significant cross-correlation (Table 3; OFC early, χ2(1) = 4.701, p = 0.030; OFC late, χ2(1) = 5.128, p = 0.024; ACC early, χ2(1) = 16.910, p < 0.001; ACC late, χ2(1) = 29.212, p < 0.001).
Effect of DOI, MK801, and amphetamine on LFP oscillations
The most consistent effect on LFP oscillations by all drugs was modulation of gamma power (Fig. 5A–L). To more accurately describe the results, we divided the gamma band into low and high ranges. In OFC, significant interactions between time and drug were detected in both low (30–55 Hz) and high (55–80 Hz) gamma bands (low gamma, F(10,52) = 7.166; high gamma, F(10,52) = 4.235; all p < 0.001). In both cases, these were driven by significant differences between drug groups during both postinjection periods but not the baseline (low gamma early bin, F(5,26) = 7.203; low gamma late bin, F(5,26) = 7.294; high gamma early bin, F(5,26) = 5.254; high gamma late bin, F(5,26) = 6.744; all p < 0.001). Similarly, in ACC there were significant interactions between time and drug detected in both low and high gamma bands (low gamma, F(10,40) = 11.999; high gamma, F(10,40) = 8.240; all p < 0.001). Both postinjection periods were marked by significant differences between groups (low gamma early bin, F(5,20) = 16.668; low gamma late bin, F(5,20) = 14.896; high gamma early bin, F(5,20) = 9.911; high gamma late bin, F(5,20) = 18.234, all p < 0.001).
The 3.0 mg/kg dose of DOI decreased OFC low and high gamma power (Fig. 6A,B; low gamma, F(2,10) = 18.624, p < 0.001; high gamma, F(2,10) = 10.479, p = 0.004). The 5.0 mg/kg dose reduced OFC low gamma (F(2,10) = 13.706, p = 0.011) but not high gamma power (Fig. 6A,B). The effect of DOI was sustained throughout the entire postinjection period in both low and high gamma bands (Fig. 6C). A similar trend was found in ACC. The 3.0 mg/kg dose significantly decreased low gamma power (Fig. 6D; F(2,8) = 9.832, p = 0.007). High gamma power was also reduced by 3.0 mg/kg in the early postinjection period (Fig. 6E; F(2,8) = 6.208, p = 0.024). At the 5.0 mg/kg dose of DOI, low and high gamma power were reduced during both postinjection periods (Fig. 6D,E; low gamma, F(2,8) = 33.340, p < 0.001; high gamma, F(2,8) = 16.580, p = 0.001). In ACC, reductions of gamma power were temporally consistent and dose dependent (Fig. 6F).
MK801 strongly increased gamma power in ACC, with less effect in OFC (Fig. 6A,B,D,E). There was a modest and nonsignificant increase in the power of low gamma activity in OFC (Fig. 6A,B). ACC gamma power was significantly increased in both low and high gamma bands (Fig. 6D,E). Amphetamine increased OFC low gamma power (Fig. 6A) and high gamma power (Fig. 6B). In ACC, high gamma power was increased more than low gamma power (Fig. 6D,E). Thus, in contrast to DOI, both amphetamine and MK801 increased gamma power.
DOI, MK801, and amphetamine reduce coupling of spike-discharge and gamma power
The correlation between changes in gamma power and single unit discharge rate was examined for all treatments in both the low and high gamma bands (Fig. 7A–D). We observed that vehicle weakly reduced the correlation between gamma power and discharge rate, while psychotomimetic drugs modulated this correlation more strongly (Fig. 7A–D). In OFC, 1.0 and 5.0 mg/kg DOI and MK801 significantly decreased mean correlations between spike-discharge and high gamma power compared with vehicle in the early postinjection period (Fig. 7B; F(5,149) = 3.057, p = 0.012, all post hoc tests p < 0.05). DOI at 5.0 mg/kg also decreased the mean correlation in the late postinjection period (F(5,149) = 2.494, p = 0.034, post hoc test p < 0.05). In ACC, more robust differences between vehicle and psychotomimetic drugs were observed. DOI (1.0 mg/kg), MK801, and amphetamine decreased discharge-low gamma power correlation in the early postinjection period (Fig. 7C; F(5,183) = 2.954, p = 0.014, all post hoc tests p < 0.05). All drugs except the lowest dose of DOI significantly reduced the ACC discharge-low gamma power correlation compared with vehicle during the late postinjection period (Fig. 7C; F(5,183) = 4.193, p = 0.001, post hoc test p < 0.05). Similarly, all drugs except the lowest dose of DOI decreased the ACC discharge-high gamma power correlation compared with vehicle (Fig. 7D; early, F(5,183) = 5.706, p < 0.001; late, F(5,183) = 5.848, p < 0.001; all post hoc tests p < 0.05).
Of note, we did not observe consistent changes in the correlation between spike-discharge and spectral power in other frequency bands (data not shown). Furthermore, we did not observe modulation of spike-field coherence by these drugs at any frequency band in either brain region (data not shown). Together, these data indicate that a common detrimental effect of different classes of psychotomimetic drugs in the PFC is to reduce the spontaneous coupling of single unit activity with gamma oscillations.
Discussion
Despite distinct pharmacological profiles, serotonergic hallucinogens, NMDA receptor antagonists, and amphetamine are all psychotomimetic in humans, and produce cognitive deficits in humans and laboratory animals. This suggests that these drugs similarly disrupt the function of brain networks that lead to aberrant behaviors related to schizophrenia. Understanding the nature of these network level disruptions may provide insight into mechanisms by which different molecular factors can lead to similar behavioral endpoints. We found that while these drugs had different inhibitory or excitatory effects on OFC and ACC population activity in awake animals, they similarly disrupted net population activity, selectively modulated LFP gamma power, and reduced the correlation of spike rate and gamma power.
Effects on single unit and population activity
The serotonergic hallucinogen DOI dose-dependently inhibited spontaneous population activity of ACC and OFC neurons. In contrast, MK801 increased population activity, and amphetamine activated or suppressed many units, thus weakly influencing population activity. While the impact of amphetamine and MK801 on PFC population activity has been reported before (Jackson et al., 2004; Homayoun and Moghaddam, 2008), this is the first investigation of the effects of serotonergic hallucinogens on cortical neurophysiology in awake animals. The lowest dose of DOI drove weak and sporadic increases in ACC single unit activity, which did not modulate population activity. Higher doses of DOI predominantly decreased the activity of individual ACC units in a sustained fashion. DOI predominantly suppressed OFC single unit activity at all doses. In contrast to MK801 and amphetamine, DOI dose-dependently decreased OFC and ACC population activity.
Our population level findings agree with previous anesthetized recordings, demonstrating reduced neuronal activity in medial PFC (including ACC) and OFC following iontophoresis of DOI (Ashby et al., 1989, 1990; Rueter et al., 2000). DOI reduces the intrinsic excitability of cortical neurons and activates inhibitory circuits, which could potentially drive these effects (Sheldon and Aghajanian, 1990; Abi-Saab et al., 1999; Zhou and Hablitz, 1999; Carr et al., 2002) (but see Ashby et al., 1990). In contrast to these studies, DOI mediates excitatory postsynaptic effects in slice preparations from prelimbic and infralimbic cortices (Aghajanian and Marek, 1997, 1999; Marek and Aghajanian, 1998b, 1999; Zhang and Marek, 2008). Thus, our results are in agreement with some previous studies, but contrast with others. This difference may be due to differential serotonergic modulation of pyramidal cell activity in PFC subregions. Previous studies reporting excitatory effects have focused mainly on rat prelimbic and infralimbic cortices, whereas inhibitory effects were observed mainly in piriform cortex, OFC, and ACC (Ashby et al., 1989, 1990; Sheldon and Aghajanian, 1990; Aghajanian and Marek, 1997, 1999; el Mansari and Blier, 1997; Marek and Aghajanian, 1998b, 1999; Rueter et al., 2000; Scruggs et al., 2000; Puig et al., 2003; Scruggs et al., 2003; Muschamp et al., 2004; Zhang and Marek, 2008). Furthermore, recordings in prelimbic and infralimbic cortices have targeted mostly cells in layer V of the PFC, whereas our data set was comprised of a more heterogeneous sample of cortical neurons. Previous reports of inhibitory effects from OFC and ACC have sampled across cortical layers as well (Ashby et al., 1989, 1990; el Mansari and Blier, 1997; Rueter et al., 2000). Collectively, these data suggest that serotonergic hallucinogens do not produce a uniform disinhibitory influence on all PFC subregions and layers. Current theories, which factor in novel mechanisms of antipsychotic drug action, suggest psychotomimetic NMDA receptor antagonists and serotonergic hallucinogens disinhibit the PFC uniformly and through a common mechanism (Aghajanian and Marek, 2000; Gray and Roth, 2007a,b; González-Maeso et al., 2008; González-Maeso and Sealfon, 2009). However, our data show that MK801 increased discharge in the same networks inhibited by DOI, suggesting that disinhibition theories of psychotomimetic states require reevaluation.
Although each drug had different effects on neuronal population activity, when the activity of each unit was absolute value transformed, equivalently sized disruptions of population activity were observed. The integrity of cortical networks depends on maintaining a delicate balance of inhibitory and excitatory neurotransmission (van Vreeswijk and Sompolinsky, 1996). Thus, excitation or inhibition produced by these drugs at any node in a neuronal network could potentially disrupt the activity of that network, leading to perceptual disorganization and cognitive deficits (London et al., 2010). Along these lines, antipsychotic efficacy may be a product of restoring network activity to self-organized levels. In support of this mechanism, antipsychotic drugs normalize both psychotomimetic drug-induced increases and decreases in neuronal discharge (Homayoun and Moghaddam, 2008). Collectively, these data suggest that the psychotomimetic effect of these drugs may arise, in part, from the decreased integrity of signaling by cortical populations.
Effects on local field potentials
In both OFC and ACC, psychotomimetic drugs modulated the power of gamma oscillations. DOI reduced gamma power, an effect which disrupts spike timing (Fuchs et al., 2007), and may engender a schizophrenia-like state by disrupting the organization of spike-discharge within neuronal networks (Uhlhaas and Singer, 2010). DOI modulated both low and high gamma power, but had a stronger effect on low gamma. On the other hand, the effects of amphetamine were larger in upper gamma band. Low and high gamma bands are pharmacologically dissociable (Oke et al., 2010) and differentially modulate PFC-dependent cognition (Wyart and Tallon-Baudry, 2008; Chaumon et al., 2009). Our data indicate that, while psychotomimetic drugs preferentially disrupt gamma power, these effects are dissociable in terms of the direction of change in gamma power as well as the frequency ranges that are impacted. Gamma oscillations are reflective of local network activity and support working memory, attention, and other aspects of human cognition affected in schizophrenia (Fries et al., 2001, 2007; Buzsáki and Draguhn, 2004; Traub et al., 2004; Womelsdorf et al., 2006; Lisman and Buzsáki, 2008; Schroeder and Lakatos, 2009; Uhlhaas and Singer, 2010). Thus, disruption of spontaneous gamma power may be indicative of, or cause, disrupted network signaling and cognitive impairments.
Spontaneous correlations between spike-rate and gamma power are associated with cognitive processing in humans and laboratory animals (Liu and Newsome, 2006; Nir et al., 2007; Denker et al., 2011). During baseline recordings in freely moving animals, we found a positive correlation between fluctuations in gamma power and neuronal discharge rate. All psychotomimetic drugs decreased this spontaneous correlation relative to vehicle or baseline, most prominently in ACC, despite the fact that they had divergent effects on population activity and gamma power. While a causal link between these correlations and the effects on population activity, gamma power modulation, or behavior has not been established, previous work suggests that both NMDA receptor antagonists and amphetamine decouple PFC gamma oscillators from their controlling networks (Pinault, 2008; Uhlhaas and Singer, 2010). It has also been suggested that decreased correlations between spike-rate and gamma power represent decoupling of a neuron's spike output from the activity of the population (Nir et al., 2007). Together, our data demonstrate that psychotomimetic drugs decouple single unit discharge from rhythmic oscillations in OFC and ACC, and thereby decrease coordination of neuronal populations. This mechanism is in line with our observation that each drug disrupted population activity to a similar degree, suggesting that the net destruction of well controlled spike-discharge and disconnection from network oscillations may be a shared outcome of these psychotomimetic drugs.
Conclusions
In freely moving animals, the serotonergic hallucinogen DOI reduced population activity and the power of gamma oscillations across PFC regions. In contrast, NMDA receptor antagonists increased population activity and gamma power. While each psychotomimetic drug produced diverse effects on the activity of individual neurons, they produced comparable levels of net disruption on population activity and decoupled single unit discharge from gamma oscillations in both PFC subregions. As opposed to disinhibition of PFC populations, disorganization of the spiking and oscillator activity in PFC networks may be common pathways through which distinct molecular factors can lead to disorganized behavior and psychosis. These findings suggest that large scale analysis of cortical activity, such as population disruptions or spike-field interactions, may provide a novel electrophysiological approach to characterize animal models of schizophrenia.
Footnotes
- Received December 21, 2011.
- Accepted December 23, 2011.
This work was supported by the National Institute of Mental Health (B.M.), the Pittsburgh Life Sciences Greenhouse (B.M.), and the Andrew Mellon Foundation for a predoctoral fellowship (J.W.).
The authors declare no competing financial interests.
- Correspondence should be addressed to Bita Moghaddam, University of Pittsburgh, Department of Neuroscience, A210 Langley Hall, Pittsburgh, PA 15260. bita{at}pitt.edu
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