Abstract
Information processing in the striatum is critical for basal ganglia function and strongly influenced by neuromodulators (e.g., dopamine). The striatum also receives modulatory afferents from the histaminergic neurons in the hypothalamus which exhibit a distinct diurnal rhythm with high activity during wakefulness, and little or no activity during sleep. In view of the fact that the striatum also expresses a high density of histamine receptors, we hypothesized that released histamine will affect striatal function. We studied the role of histamine on striatal microcircuit function by performing whole-cell patch-clamp recordings of neurochemically identified striatal neurons combined with electrical and optogenetic stimulation of striatal afferents in mouse brain slices. Bath applied histamine had many effects on striatal microcircuits. Histamine, acting at H2 receptors, depolarized both the direct and indirect pathway medium spiny projection neurons (MSNs). Excitatory, glutamatergic input to both classes of MSNs from both the cortex and thalamus was negatively modulated by histamine acting at presynaptic H3 receptors. The dynamics of thalamostriatal, but not corticostriatal, synapses were modulated by histamine leading to a facilitation of thalamic input. Furthermore, local inhibitory input to both classes of MSNs was negatively modulated by histamine. Subsequent dual whole-cell patch-clamp recordings of connected pairs of striatal neurons revealed that only lateral inhibition between MSNs is negatively modulated, whereas feedforward inhibition from fast-spiking GABAergic interneurons onto MSNs is unaffected by histamine. These findings suggest that the diurnal rhythm of histamine release entrains striatal function which, during wakefulness, is dominated by feedforward inhibition and a suppression of excitatory drive.
Introduction
The basal ganglia and particularly the input layer of the basal ganglia, the striatum, play a critical role in the control of motor behavior and cognitive function (Graybiel et al., 1994; Grillner et al., 2005; Yin and Knowlton, 2006). The main computational unit of the striatum is the GABAergic medium spiny projection neuron (MSN) of which there are at least two classes; the dopamine receptor 1 (D1)-expressing and dopamine receptor 2 (D2)-expressing MSNs which correspond to the direct and indirect pathway neurons respectively (Gerfen et al., 1990; Smith et al., 1998). Both classes of MSN receive and integrate cortical and thalamic excitatory input (Kincaid et al., 1998; Lacey et al., 2007; Doig et al., 2010) and selectively innervate downstream basal ganglia nuclei and differently affect motor behavior (Kravitz et al., 2010). Their activity is controlled by local GABAergic and cholinergic interneurons (Kawaguchi et al., 1995; Mallet et al., 2005), reciprocal inhibitory connections between neighboring MSNs (Tepper and Plenz, 2006) and neuromodulators such as dopamine (Schultz, 2002; Ungless, 2004; Surmeier et al., 2007), serotonin (Steinbusch, 1981; Mathur et al., 2011; Parent et al., 2011) and noradrenaline (Aston-Jones and Bloom, 1981).
The striatum also receives input from histaminergic neurons located in the tuberomamillary nucleus of the hypothalamus (Haas and Panula, 2003). Histaminergic neurons exhibit a diurnal rhythm in their activity, being active during wakefulness, especially during periods of increased attention (Takahashi et al., 2006), and relatively inactive or silent during sleep (Reiner and McGeer, 1987; Steininger et al., 1999; Takahashi et al., 2006). Recent studies using knock-out animals have suggested they play a role in mediating specific aspects of wakefulness (Parmentier et al., 2002; Anaclet et al., 2009). The striatum also displays a high density of histamine receptors (Hill and Young, 1980; Martinez-Mir et al., 1990; Vizuete et al., 1997; Pillot et al., 2002) suggesting that released histamine has the potential to exert widespread effects on striatal function. Indeed, it has been shown that histamine can modulate corticostriatal transmission in both rats and mice (Doreulee et al., 2001) and the intrinsic properties of striatal neurons (Munakata and Akaike, 1994).
The aim of this investigation was thus to define the role of histamine in controlling the activity of the striatal network. To achieve this aim we performed whole-cell patch-clamp recordings of identified D1- or D2-expressing MSNs in mouse brain slices and determined the effect of histamine on the membrane potential, excitatory afferents from the cortex and thalamus and local GABAergic input to MSNs. We further characterized the effects on GABAergic inputs by using dual whole-cell patch-clamp recordings, investigating the effects of histamine on the unitary connections between fast-spiking GABAergic interneuron–MSN and MSN–MSN pairs. We find that histamine suppresses the excitatory drive to MSNs, selectively alters the short-term dynamics of thalamostriatal synapses and abolishes feedback inhibition onto MSNs.
Materials and Methods
Animals.
All experiments were performed on transgenic mouse lines of either sex which were bred and housed in accordance with the Animals (Scientific Procedures) Act (1986) and the Society of Neuroscience policy on the use of animals in neuroscience research. The majority of the recordings were performed on BAC transgenic mice that report subtypes of the dopamine receptor, either D1 or D2, by the presence of GFP (Mutant Mouse Regional Resource Centers, MMRRC). Details of the mice and the methods of BAC mice production have been published (Gong et al., 2003) and can be found on the GENSAT website [GENSAT (2009) The Gene Expression Nervous System Atlas (GENSAT) Project. In: NINDS, Contracts N01NS02331 and HHSN271200723701C, The Rockefeller University (New York), http://www.gensat.org/index.html]. Lhx6-GFP mice report a subset of GABAergic interneurons and were obtained from the MMRRC and kept as a heterozygous breeding line on a Swiss Webster background. CaMKII-cre mice express cre recombinase in all CaMKII-expressing neurons and were obtained from the Jackson Laboratory and kept as a homozygous breeding line.
Slice preparation.
Oblique coronal striatal slices (300–400 μm) were prepared from postnatal day 18–35 D1-GFP, D2-GFP, or Lhx6-GFP mice or, for optogenetic experiments, 1- to 4-month-old injected CaMKII-cre mice. Slices were taken between ∼+1.60 mm and −1.30 mm from bregma. Mice were anesthetized with isoflurane and decapitated. Slices were prepared in artificial CSF (ACSF) containing the following (in mm): 130 NaCl, 3.5 KCl, 1.25 NaH2PO4, 5 MgCl2, 2.5 CaCl2, 24 NaHCO3, and 10 glucose, pH 7.2–7.4, bubbled with carbogen gas (95% O2/5% CO2). Slices were immediately transferred to a storage chamber containing ACSF (in mm): 130 NaCl, 3.5 KCl, 1.25 NaH2PO4, 1.5 Mg Cl2, 2.5 CaCl2, 24 NaHCO3, and 10 glucose, pH 7.2–7.4, bubbled with carbogen gas, at 37°C for 30 min and subsequently maintained at room temperature until used for recording.
Recording.
Whole-cell current-clamp and voltage-clamp recordings from single or pairs of dorsal striatal neurons were performed using glass pipettes, pulled from standard wall borosilicate glass capillaries containing the following: for whole-cell current-clamp (in mm), 110 potassium gluconate, 40 HEPES, 2 ATP-Mg, 0.3 Na-GTP, 4 NaCl, and 4 mg/ml biocytin, pH 7.2–7.3 (osmolarity, 290–300 mOsm/L); and for whole-cell voltage-clamp (in mm), 120 cesium gluconate, 40 HEPES, 4 NaCl, 2 ATP-Mg, 0.3 Na-GTP, 0.2 QX-314, and 4 mg/ml biocytin, pH 7.2–7.3 (osmolarity, 290–300 mOsm/L). Paired recordings of fast-spiking GABAergic interneuron (FSI)–MSN and MSN–MSN connected pairs were made using a high chloride concentration intracellular solution containing the following (in mm): 105 potassium gluconate, 30 KCl, 10 HEPES, 4 ATP-Mg, 0.3 Na-GTP, and 4 mg/ml biocytin (pH 7.2–7.3; osmolarity, 290–300 mOsm/L). All recordings were made using HEKA amplifiers with integrated A/D converter and acquired using Pulse or Patchmaster software (HEKA Electronik).
Stimulation and recording protocols.
MSN afferents were stimulated electrically or optically. Electrical stimulation was performed by placing a glass stimulating electrode in the external capsule for activation of corticostriatal afferents, or for activation of inhibitory fibers at 100–200 μm from the patched MSN soma. Stimulation strength was set to evoke ∼1/3 of maximum response corresponding to a stimulation strength of 100–300 μA. Optical stimulation of corticostriatal and thalamostriatal afferents was performed using the optoLED system (Cairn Research), consisting of a 470 nm, 3.5 W LED mounted on a Zeiss Axioskop 2 FS microscope, to give 3 ms duration light pulses of ∼5% of maximum output power. The spot size corresponded to the area of the slice visualized using a 40×/0.8 numerical aperture water-immersion objective. Activation of excitatory afferents was performed in the presence of blockers of inhibitory GABAergic transmission including the GABAA receptor antagonist SR95331 (10 μm) and GABAB receptor antagonist CGP52432 (2 μm). Activation of inhibitory afferents was performed in the presence of blockers of excitatory transmission including the NMDA receptor antagonist d-AP5 (50 μm) and AMPA/kainate receptor antagonist NBQX (20 μm). Fibers were activated every 10 s and EPSCs or IPSCs were recorded in the patched MSN. Evoked EPSCs and IPSCs were recorded in whole-cell voltage-clamp mode at a holding potential respectively near −80 mV and 0 mV (estimated reversal potential for glutamatergic transmission). For paired pulse stimulation, two stimulating pulses were consecutively given at 50 ms interval and repeated every 10 s for up to 20 times. Trains of pulses consisted of 9 pulses at 20 Hz followed by a recovery pulse 500 ms later, and was repeated every 30 s for up to 5 times. Baseline responses were measured for 5 min after which histamine, alone or in combination with histamine receptor antagonists, was washed in for 10 min, followed by a 10 min washout. Dose–response experiments were performed using 10 min exposures to increasing concentrations of histamine (1, 5 and 10 μm). Recording of MSN resting membrane potential was performed in whole-cell current-clamp mode. If the resting membrane potential of the patched neuron exhibited a stable baseline for 5 min (<5% change) histamine, alone or in combination with histamine receptor antagonists, was washed in for 10 min, followed by a 10 min washout while the membrane voltage was constantly monitored. Paired recordings were performed by evoking a single action potential in the presynaptic neuron using a suprathreshold current injection and recording the unitary IPSC (uIPSC) as an inward current from the postsynaptic neuron held near −80 mV.
Viral transfection.
Adeno-associated virus serotype 2 (AAV2) carrying fusion genes for channelrhodopsin 2 (ChR2) and yellow fluorescent protein (YFP) were injected into the thalamus or cortex of CaMKII-cre mice between postnatal days 14 and 21. For thalamostriatal experiments, the intralaminar nuclei of the thalamus were targeted. For corticostriatal experiments, layers II/III of the cortex were targeted. Typical coordinates from bregma for thalamic injections were lateral, 0.7 mm; posterior, 1.6 mm; and 3.1 mm ventral to the surface of brain. For cortical injections the coordinates were lateral, 0.7 mm; posterior, 0.1 mm; and 0.3 mm ventral to the surface of brain. Viral DNA included the double-floxed sequence for ChR2(H134R)-EYFP driven by the elongation factor 1 promotor. AAV2 particles were produced at the University of North Carolina Gene Therapy Center Virus Vector Core. Typical titers were ∼1012 IU/ml. Injection volumes were 300–400 nl. After allowing 3–14 weeks for ChR2-YFP expression, acute striatal slices were prepared as described above.
Analysis of intracellular recordings.
Data were analyzed offline using custom written procedures in Igor Pro (Wavemetrics). PSCs were detected as upward or downward deflections of >2 SDs above baseline. Paired pulse ratios were calculated by dividing the average slope of the second PSC with the average slope of the first PSC. Slopes of individual PSCs were determined between 20–80% of maximum PSC amplitude. Trains were analyzed by taking the amplitude of each PSC and dividing this by the amplitude of the first PSC. To extract correct amplitudes of postsynaptic responses lying on the decay phase of previous responses, the synaptic decay was fitted by an exponential curve and subtracted. For the MSN–MSN paired recordings the amplitudes of every three evoked uIPSCs were averaged due to the small amplitude responses and failures at these synapses. The input resistance was calculated from the slope of a line fitted to the injected current versus the steady-state membrane voltage when a family of hyperpolarizing and depolarizing current injections were applied (range, −300/+600 pA). The analysis of EPSC kinetics (peak amplitude, duration, rise time (20–80%), half maximum peak, half decay time and time to peak) was performed on individual synaptic responses. Failure rate was calculated for individual pairs as the number of failures divided by the total number of stimulations and averaged over pairs.
Histological analyses.
Following intracellular recording, the slices were fixed overnight in 4% paraformaldehyde and 15% saturated picric acid in 0.1 m phosphate buffer (PB; pH 7.4) at 4°C. Slices were embedded in 5% agar and resectioned at 50 μm on a vibrating microtome (VT1000S; Leica Microsystems). Autofluorescence was reduced by incubating the sections in 1% sodium borohydride in PBS for 10 min at room temperature. All sections were preincubated with 10–20% normal donkey serum (NDS; Vector Laboratories) in PBS for >1 h at room temperature. Biocytin-filled cells were visualized by incubating sections in 1:1000 streptavidin-Cy3 conjugate (ZyMax; Invitrogen) or 1:10,000 streptavidin-405 conjugate (Invitrogen) in PBS containing 0.3% Triton-X (PBS-Tx) overnight at 4°C. GFP expression was confirmed for MSNs recorded from slices of D1- and D2-GFP mice and FSIs from Lhx6-GFP mice by incubating sections in 1:400 rabbit anti-GFP-Alexa Fluor 488 conjugate (Invitrogen) in PBS-Tx or in 1:1000 chicken anti-GFP (Aves Labs) in PBS-Tx and 1% NDS overnight at 4°C followed by 1:500 donkey-anti-chicken-Alexa Fluor 488 fluorophore (Jackson ImmunoResearch Laboratories) in PBS-Tx for 2 h at room temperature. To define the subtype of MSN in recordings performed in CaMKII-cre mice, the sections were heated at 80°C in 10 mm sodium citrate, pH 6.0, for ∼30 min before incubation with 1:1000 rabbit anti-preproenkephalin (LifeSpan Biotechnology) in PBS-Tx and 1% NDS overnight at 4°C after which the reaction was revealed by incubating with donkey-anti-rabbit-Cy3 fluorophore (Jackson ImmunoResearch Laboratories) in PBS-Tx for 2 h at room temperature. The neurons that were immunopositive were classified as D2 or indirect pathway MSNs.
Histamine fibers were visualized in perfusion-fixed tissue of D1- or D2-GFP transgenic mice. The mice were transcardially perfused with 50 ml of ice-cold 0.1 m PB, pH 7.4, followed by ice-cold 4% 1-ethyl-3-[3-dimethylaminopropyl] carbodiimide HCl (Thermo Fisher Scientific) in 0.1 m PB, pH 7.4. The brains were removed and immersed in the same fixative for 3 d followed by 3% paraformaldehyde in 0.1 m PB for 1 d. Sagittal vibratome sections (40 μm) were collected and treated with a solution of 0.5% sodium borohydride for 30 min. After rinsing, the sections were incubated with 10% normal goat serum in PBS-Tx for 2 h and double-immunolabeled to reveal GFP and histamine. Sections were incubated in 1:50,000 rabbit-anti-histamine (Immunostar) together with 1:1000 chicken-anti-GFP (Aves Labs) for at least 72 h at 4°C. After this, sections were washed and incubated overnight at 4°C in a mixture of 1:500 biotinylated goat-anti-rabbit IgG (Vector Laboratories) and 1:100 goat-anti-chicken-Alexa Fluor 488 fluorophore (Invitrogen) secondary antibodies. The sections were then washed and incubated in ABC Elite (Vector Laboratories) for 4 h at room temperature after which the signal was amplified using 1:100,000 biotinylated tyramide in 50 mm PBS, pH 7.4 (see for detailed procedure (Kuramoto et al., 2009). Sections were washed thoroughly and then incubated overnight at 4°C in 1:1500 anti-streptavidin-Cy3 fluorophore (ZyMax, Invitrogen).
To confirm the AAV injection were correctly targeted to the thalamic intralaminar nuclei 50 μm sections were made from paraformaldehyde-fixed brains (4% in 0.1 m PB) of injected CaMKII-cre mice used for experiments. Sections were incubated in 20% NDS (Vector Laboratories) for 45 min at room temperature. YFP was visualized by immunolabeling using 1:1000 chicken-anti-GFP (Aves Labs) in PBS-Tx and 1% NDS overnight at 4°C followed by 1:500 donkey-anti-chicken-Alexa Fluor 488 fluorophore (Jackson ImmunoResearch Laboratories) in PBS-Tx for 2 h at room temperature. To facilitate anatomical characterization the sections were incubated for 30 min in a 1:200 Nissl-Cy5 stain (Neurotrace, Invitrogen).
Additional double-labeling immunohistochemical experiments were performed on paraformaldehyde-fixed (4% in 0.1 m PB) sections from D1- and D2-GFP mice, to compare the pattern of innervation by histaminergic fibers versus the pattern of innervation provided by the dopaminergic, glutamatergic and GABAergic systems, to direct and indirect pathway MSNs in the striatum. Incubations were performed with 1:1000 chicken-anti-GFP (Aves Labs), together with 1:1000 rabbit-anti-tyrosine hydroxylase (Millipore) antibody, 1:2000 rabbit-anti-vesicular glutamate transporter type 1 (VGluT1) (Mabtech), 1:2000 rabbit-anti-vesicular glutamate transporter type 2 (VGluT2) (Synaptic Systems) or 1:2000 guinea pig-anti-vesicular GABA transporter (VGAT) (Synaptic Systems) antibodies. This was followed by incubation in a mixture of 1:500 donkey-anti-chicken-Alexa Fluor 488 fluorophore (Jackson ImmunoResearch) together with 1:500 donkey-anti-rabbit-Cy3 fluorophore (Jackson ImmunoResearch) or 1:300 donkey-anti-guinea pig-Cy5 fluorophore (Jackson ImmunoResearch) secondary antibodies.
Finally, all sections were mounted in Vectashield (Vector Laboratories) and images were captured with a LSM 710 (Zeiss) confocal microscope using ZEN and Axiovison software (Zeiss). The software's default settings for fluorophores were used for beamsplitters and ranges of emissions sampled.
Statistics.
All data are presented as means ± SEM, except where stated. Student's t tests and repeated-measures ANOVA were performed using SPSS 17.0 (*p < 0.05, **p < 0.01).
Drugs and chemicals.
All drugs were obtained from Tocris Bioscience and Sigma-Aldrich.
Results
The striatum receives a sparse histaminergic innervation
We first investigated the presence of histamine fibers in the D1 and D2 BAC transgenic mice which report the subtype of dopamine receptor by the presence of GFP. Using a polyclonal antibody against histamine we found histamine-expressing neurons only in the tuberomamillary nucleus of the hypothalamus (Fig. 1A) consistent with findings in other species (Airaksinen and Panula, 1988; Inagaki et al., 1988). We found that different areas of the brain of D1- and D2-GFP mice had different densities of histaminergic innervation. The striatum was sparsely innervated by histamine-positive fibers that often traversed the striatum in the ventrodorsal plane and possessed prominent varicosities (Fig. 1B). This sparseness was especially apparent when compared with dopaminergic innervation of the striatum revealed by tyrosine hydroxylase immunostaining (Fig. 1C). The sparseness of innervation was also evident when compared with glutamatergic excitatory input from the cortex as revealed by VGluT1 immunostaining (Fig. 1D), glutamatergic excitatory input from the thalamus as revealed by VGluT2 immunostaining (Fig. 1E) and GABAergic innervation as revealed by VGAT immunostaining (Fig. 1F). Despite this sparse innervation the striatum has been reported to have a high density of histamine receptors (Hill and Young, 1980; Martinez-Mir et al., 1990; Vizuete et al., 1997; Pillot et al., 2002). Furthermore, since no specific transporter of histamine has been described (Haas and Panula, 2003), histamine, once released, could have widespread effects on striatal function. We thus determined the effect of histamine on the intrinsic properties of MSNs and both the excitatory and inhibitory inputs to MSNs.
Cortical excitatory input to MSNs is negatively modulated by histamine acting at the H3 receptor
First, we investigated whether the glutamatergic input from the cortex to the different classes of MSN is modulated by histamine. A stimulating electrode was placed in the external capsule and cortical afferents were activated at 10 s intervals while recording EPSCs in whole-cell voltage-clamp mode from direct and indirect pathway MSNs in D1- and D2-GFP mice. All the experiments were performed in the presence of the GABAA receptor antagonist SR95331 (10 μm) and the GABAB receptor antagonist CGP52432 (2 μm). A 5 min baseline response was recorded after which histamine (10 μm) was washed in for 10 min, followed by 10 min washout. The concentration of histamine was chosen in accordance with previous studies (Brown and Haas, 1999; Atzori et al., 2000; Doreulee et al., 2001) that demonstrated this to be an effective concentration to study histamine in vitro. For all electrophysiological experiments using the D1- and D2-GFP transgenic mice the MSN subtype was confirmed post hoc by immunolabeling for GFP (Fig. 2A,B). We recorded from a total of 25 MSNs (consisting of >80% GFP-positive neurons) in the dorsal striatum (Fig. 2Ci).
We observed a depression of cortically evoked glutamatergic transmission in response to wash-in of histamine in both D1 and D2 MSNs to 70–80% of baseline (Fig. 2Cii, D1: 81.8 ± 6.6% and D2: 71.0 ± 10.0%; both p < 0.05; paired samples t test; n = 13 and n = 12). There was no significant difference in the histaminergic-mediated depression between D1 and D2 MSNs (p > 0.05; n = 13 and n = 12). The decrease in EPSC amplitude was blocked by coapplication of the histamine 3 (H3) receptor antagonist, thioperamide (10 μm) (Fig. 2Ciii, D1: 105.0 ± 9.4%; p < 0.05 and D2: 113.4 ± 8.8%; p < 0.01; independent samples t test; n = 11 and n = 7). Washout of histamine for 10 min was not sufficient to reverse the depression of cortically evoked glutamatergic transmission (Fig. 2Cii), consistent with previous reports (Brown and Haas, 1999; Doreulee et al., 2001). However, we found that the negative modulation of glutamatergic transmission by histamine could be reversed by the application of thioperamide (to 102.0 ± 9.4%; p < 0.05; paired samples t test; n = 4). Thioperamide alone did not affect the EPSC amplitude (Fig. 2Ciii, D1: 95.8 ± 12.8% and D2: 93.4 ± 13.0%; both p > 0.05; independent samples t test; n = 4 and n = 5). Last, we investigated whether lower concentrations of histamine (1 and 5 μm) affect corticostriatal transmission. We found that histamine at 1 μm concentration already leads to a significant decrease in EPSC amplitude (to 86.7 ± 1.6%; p < 0.01; paired samples t test; n = 6), with a near maximal decrease at 5 μm (5 μm: to 62.9 ± 5.0% and 10 μm: to 59.2 ± 6.3%; p > 0.05; paired samples t test) consistent with previous observations (Doreulee et al., 2001). These results suggest that histamine negatively modulates cortical excitatory inputs to both classes of MSN by acting at H3 receptors.
Thalamic excitatory input to MSNs is negatively modulated by histamine acting at the H3 receptor
We next investigated whether thalamic glutamatergic input to the different classes of MSN is modulated by histamine. To avoid antidromic activation of cortical inputs and activation of fibers of passage from other brain regions we used an optogenetic approach to isolate thalamic afferents (see Materials and Methods). In brief, the thalamic intralaminar nuclei of CaMKII-cre mice were injected with AAV2 containing the double-floxed sequence for the light activatable ion channel ChR2 and YFP (Fig. 3A). After a survival time of 3–14 weeks, brain slices were prepared as described above. The survival time enables sufficient expression of ChR2 throughout the axonal arbor of the thalamic neurons including their projection to the striatum. Fluorescence illumination of the striatum in these brain slices reveals a dense network of YFP-positive fibers (Fig. 3B,C). Whole-cell voltage-clamp recordings of striatal MSNs were performed while activating the thalamic afferents by illuminating the striatum with brief light pulses (470 nm; 3 ms duration). The subtype of MSN was confirmed post hoc by immunolabeling for preproenkephalin (PPE) which is selectively expressed by the D2 (presumed indirect pathway) MSNs (Gerfen et al., 1990) (Fig. 3B). If a recorded neuron was negative for PPE it was defined as an MSN on the basis of the somatodendritic morphology and considered a D1 (presumed direct pathway) MSN.
Recordings were made from a total of 27 neurons in the dorsal striatum, located close to YFP-expressing thalamic fibers and which all exhibited an excitatory response upon brief illumination (470 nm; 3 ms duration) of the striatum (Fig. 3Ci). The optically evoked EPSCs exhibited similar amplitudes, duration and short-term dynamics to those described previously using conventional electrical stimulation of thalamic afferents (Ding et al., 2008). Wash-in of histamine reduced the amplitude of the evoked thalamic EPSCs in both PPE− and PPE+ neurons (Fig. 3Cii, PPE−: to 43.9 ± 3.9% and PPE+: to 51.7 ± 9.5%; both p < 0.01; paired samples t test; n = 5 and n = 7). There was no significant difference in the histaminergic-mediated depression between PPE− and PPE+ MSNs (p > 0.05; n = 5 and n = 7). A small number of neurons could not be classified as PPE− or PPE+ following the immunolabeling, but as a group they also exhibited a similar reduction in EPSC amplitude (to 42.8 ± 6.1%; p < 0.01; paired samples t test; n = 5). The decrease in EPSC amplitude was blocked by coapplication of the H3 receptor antagonist thioperamide (Fig. 3Ciii, PPE−: to 85.6 ± 5.8%; p < 0.05 and PPE+: to 110.0 ± 8.0%; p < 0.01; independent samples t test; n = 4 and n = 2). Thioperamide alone did not affect the EPSC amplitude (Fig. 3Ciii, PPE−: to 89.1 ± 9.1% and PPE+: to 96.9 ± 9.7%; both n = 2).
To make a direct comparison of evoked responses seen with electrical and optical stimulation, and to exclude the possibility that the observed histaminergic modulation of cortically evoked EPSCs could be the result of contamination by erroneous electrical activation of thalamic fibers, we repeated the cortical stimulation experiments but this time optogenetically (see Materials and Methods). Similar to electrically evoked EPSCs we observed a decrease in the amplitude of optically evoked cortical EPSCs in response to histamine (to 58.2 ± 8.2%; p < 0.05; paired samples t test; n = 7). The decrease in EPSC amplitude was not significantly different from that observed using electrical stimulation (p > 0.05; independent samples t test; n = 24 and n = 7), neither were any of the measured characteristics of electrical and optical evoked EPSCs significantly different (Table 1, all p > 0.05; independent samples t test; n = 7 and n = 27). Last, the decrease in optically evoked cortical EPSC amplitude was also similar to that seen for the optically evoked thalamic EPSCs (p > 0.05; independent samples t test; n = 17 and n = 7).
In conclusion, these results suggest that excitatory thalamic input to both classes of MSN, similar to that found for the excitatory cortical input, is negatively modulated by histamine acting at H3 receptors.
Histamine selectively modulates the short-term dynamics of thalamostriatal synapses
Next, we determined whether histamine is acting presynaptically or postsynaptically at the H3 receptor on cortical and thalamic afferents using a paired pulse stimulation protocol. A change in the paired pulse ratio (PPR) would suggest histamine is acting presynaptically (Thomson, 2000). MSNs were recorded in whole-cell voltage-clamp mode while cortical or thalamic afferents were activated using a paired pulse stimulation protocol consisting of two pulses given at 50 ms interval.
We found that the baseline PPR of corticostriatal synapses is facilitating (Fig. 4A, D1: 1.1 ± 0.1 and D2: 1.1 ± 0.1; n = 18 and n = 12), consistent with previous observations (Ding et al., 2008). Histamine slightly increased the PPR for both classes of MSN (Fig. 4A, D1: to 1.2 ± 0.1; p > 0.05 and D2: to 1.3 ± 0.1; p < 0.05; paired samples t test; n = 18 and n = 12) in a thioperamide-sensitive manner (Fig. 4A, D1: 1.2 ± 0.1 and D2: 1.2 ± 0.1; n = 7 and n = 5). In contrast to corticostriatal synapses the baseline PPR of thalamostriatal synapses was depressing (Fig. 4C, PPE−: 0.7 ± 0.1 and PPE+: 0.9 ± 0.1; n = 8 and n = 9), consistent with previous observations (Ding et al., 2008). However, the PPR increased and became significantly facilitating in the presence of histamine (Fig. 4C, PPE−: to 1.3 ± 0.4 and PPE+: to 2.0 ± 0.6; both p < 0.05; independent samples t test; n = 5 and n = 6) in a thioperamide-sensitive manner (Fig. 4C, PPE−: 0.8 ± 0.3 and PPE+: 1.0 ± 0.2; n = 2 and n = 3). These results demonstrate that histamine tends to increase the PPR at both corticostriatal and thalamostriatal synapses suggesting that histamine acts presynaptically at H3 receptors.
To investigate the short-term dynamics at these synapses in more detail, cortical and thalamic afferents were stimulated with trains of pulses consisting of nine pulses at 20 Hz including a recovery pulse 500 ms later. Consistent with previous findings (Ding et al., 2008) corticostriatal synapses exhibited a short-term facilitation followed by a constant depressed response (Fig. 4B, black trace), whereas thalamostriatal synapses exhibited a constant depressed response from the first pulse onwards (Fig. 4D, black trace). Interestingly, we found that histamine selectively affected corticostriatal or thalamostriatal synapses. Whereas histamine did not lead to a transition in the dynamics of corticostriatal synapses (Fig. 4B, red trace; baseline vs histamine; p > 0.05, ANOVA, n = 6 and n = 4), the thalamostriatal synapses became significantly facilitatory throughout (Fig. 4D, red trace; baseline vs histamine; p < 0.01, ANOVA; n = 17 and n = 13) in a thioperamide-sensitive manner (Fig. 4D, gray trace; n = 2).
These results suggest that histamine acts at presynaptic H3 receptors at both corticostriatal and thalamostriatal synapses. Furthermore, it suggests that histamine selectively alters the short-term dynamics of thalamostriatal synapses from depressing to facilitatory.
Histamine depolarizes both classes of MSN
The ability of cortical and thalamic excitatory inputs to initiate action potentials in a postsynaptic MSN will be dependent on the membrane voltage of the MSNs. We therefore determined whether histamine affected the resting membrane potential of MSNs using whole-cell current-clamp recordings of MSNs from D1- and D2-GFP mice (Fig. 5A). The resting membrane potential of both classes of MSN was near −80 mV (D1: −79.1 ± 2.6 mV and D2: −79.4 ± 1.0 mV; n = 10 and n = 11). Bath application of histamine significantly depolarized both classes of MSN (Fig. 5B, D1: to −72.7 ± 2.6 mV and D2: to −72.0 ± 2.2 mV; both p < 0.01 paired samples t test; n = 10 and n = 11) and led to a decrease in input resistance (baseline: 71.6 MΩ and histamine: 66.5 MΩ; p < 0.05; paired samples t test; n = 12). Next, histamine was coapplied with either the histamine 1 (H1) receptor antagonist, trans-triprolidine (2 μm), or the histamine 2 (H2) receptor antagonist, ranitidine (5 μm), to investigate which histamine receptor was responsible for the observed depolarization. Coapplication with the H1 receptor antagonist did not block the histamine-mediated depolarization (Fig. 5B, D1: from −78.0 ± 2.4 to −74.2 ± 2.5 mV; p < 0.01 and D2: from −77.0 ± 1.6 to −72.1 ± 2.9 mV; p < 0.05; paired samples t test; n = 10 and n = 11), whereas coapplication with the H2 receptor antagonist did significantly block the depolarization (Fig. 5B, D1: from −82.4 ± 1.1 to −79.4 ± 2.4 mV and D2: from −78.7 ± 1.2 to −78.2 ± 0.4 mV; both p > 0.05; paired samples t test; n = 6 and n = 4) as well as the decrease in input resistance (baseline: 76.6 MΩ and histamine + ranitidine: 78.5 MΩ; p > 0.05; paired samples t test; n = 10). These results suggest that histamine depolarizes both classes of MSN by acting at H2 receptors.
Striatal GABAergic input to MSNs is negatively modulated by histamine
The likelihood of a MSN to initiate an action potential is not only dependent on the excitatory drive and resting membrane potential, but also on the timing and strength of its inhibitory inputs derived from local collaterals of neighboring MSNs (Somogyi et al., 1981; Plenz, 2003; Tepper et al., 2004) and GABAergic interneurons (Kawaguchi et al., 1995; Mallet et al., 2005). We therefore determined the effect of histamine on inhibitory inputs to MSNs. The first approach was to place a stimulating electrode in the striatum at 100–200 μm from the recorded MSN to activate all striatal fibers, most likely consisting of afferents from both MSNs and interneurons. Afferents were activated at 10 s intervals and evoked IPSCs were recorded in whole-cell voltage-clamp as an outward current from MSNs in D1- and D2-GFP transgenic mice (Fig. 6A). All further experiments were performed in the presence of the NMDA receptor antagonist d-AP5 (50 μm) and the AMPA/kainate receptor antagonist NBQX (20 μm).
Bath application of histamine led to a marked reduction in IPSC amplitude in both populations of MSNs (Fig. 6B, D1: to 59.5 ± 5.7% and D2: to 40.2 ± 1.2%; p < 0.01; paired samples t test; n = 13 and n = 8). There was no significant difference in the histaminergic-mediated depression between D1 and D2 MSNs (p > 0.05; n = 13 and n = 8). Coapplication of the H3 receptor antagonist thioperamide completely blocked the histamine-mediated reduction in IPSC amplitude in D2 MSNs (Fig. 6C, to 103.7 ± 11.4%; p < 0.01; independent samples t test; n = 5). However, for the population of D1 MSNs, coapplication of the H3 receptor antagonist, only partially, albeit significantly, blocked the reduction in IPSC (Fig. 6C, histamine: 59.5 ± 5.7% vs histamine + thioperamide: 79.0 ± 7.0%; p < 0.05 and baseline vs histamine + thioperamide: p < 0.05; independent samples t test; n = 13 and n = 17). Thioperamide alone did not affect the IPSC amplitude (Fig. 6C, D1: to 100.7 ± 12.7% and D2: to 103.1 ± 12.0%; both p > 0.05; independent samples t test; both n = 4).
To further investigate how histamine modulates GABAergic inputs onto D1 MSNs we coapplied histamine with either the H1 receptor antagonist, trans-triprolidine (2 μm), or the H2 receptor antagonist, ranitidine (5 μm). Coapplying histamine with the H1 receptor antagonist did not affect the histaminergic modulation of IPSC amplitude (Fig. 6C, to 65.0 ± 8.8%; p > 0.05; independent samples t test; n = 13 and n = 10). However, coapplication of histamine with the H2 receptor antagonist significantly blocked part of the histaminergic modulation (Fig. 6C, to 78.0 ± 6.4%; p < 0.05; independent samples t test; n = 13 and n = 9). To conclude, these results suggest histamine strongly attenuates GABAergic transmission onto both classes of MSN by acting at H3 receptors for synapses onto D2 MSNs and at both H3 and H2 receptors for synapses onto D1 MSNs.
Feedforward inhibition is not modulated by histamine
Two major sources of GABAergic input to MSNs are the local collaterals of neighboring MSNs mediating feedback or lateral inhibition and the FSIs mediating feedforward inhibition. To investigate the contribution of each of these to the observed histaminergic modulation of GABAergic transmission we performed dual whole-cell patch-clamp recordings of connected FSI–MSN and MSN–MSN pairs.
First, we determined the effect of histamine on feedforward inhibition by performing paired recordings of connected pairs of FSIs and MSNs in Lhx6 transgenic mice, in which a subset of GABAergic interneurons express GFP (Fig. 7A,B). Both the spiking pattern of the recorded neurons to depolarizing current steps (Fig. 7A) and post hoc immunolabeling for parvalbumin (PV) and GFP (Fig. 7B) were used to determine FSI phenotype. Recordings were made from 10 pairs of FSIs and MSNs, of which, six were unidirectionally connected and in which a single action potential in the presynaptic FSI elicited a uIPSC in the MSN. A presynaptic action potential was elicited at 10 s intervals and, following a 5 min baseline recording, histamine was applied for 10 min, followed by a 10 min washout. We found that the uIPSC amplitude was not significantly affected by the histamine application (Fig. 7C, to 92.7 ± 11.7%; p > 0.05; paired samples t test; n = 6) and neither was the failure rate (baseline: 0.2 ± 0.1 and histamine: 0.3 ± 0.1).
To investigate whether the short-term dynamics at this synapse was modulated by histamine we used paired pulse and train stimulation protocols. Paired pulse stimulation consisted of two action potentials at a 50 ms interval elicited in the presynaptic FSI and train stimulation consisted of nine action potentials at 20 Hz followed by a final action potential 500 ms later (Planert et al., 2010). Both the baseline PPR (0.67 ± 0.02; n = 4) and the response to train stimulation throughout the 20 Hz train was depressing, consistent with previous reports (Gittis et al., 2010; Planert et al., 2010). Application of histamine did not affect the depressed response in the PPR (0.6 ± 0.2; p > 0.05; paired samples t test; n = 4) nor the depressed response to train stimulation (p > 0.05; ANOVA; n = 5). Combined, these results suggest that neither the GABAergic transmission or short-term dynamics between FSIs and MSNs is modulated by histamine.
Feedback inhibition between MSNs is negatively modulated by histamine
Next, we investigated whether histamine modulates lateral inhibition between neighboring MSNs by using dual whole-cell patch-clamp recordings of connected pairs of MSNs in D1- and D2-GFP transgenic mice (Fig. 7D,E). Recordings were made from forty-four pairs of MSNs of which five were unidirectionally connected (Fig. 7F), and in which a single action potential in the presynaptic MSN elicited a uIPSC in the postsynaptic MSN. The connection probability was consistent with ∼10% connectivity as previously observed in vitro (Planert et al., 2010). A presynaptic action potential was elicited every 10 s, and following a 5 min baseline recording, histamine was applied for 10 min, which was followed by a 10 min washout. Histamine application abolished all uIPSCs between all the recorded pairs of MSNs (Fig. 7F, n = 5). The absence of any detectable uIPSCs was not the result of an inability to elicit presynaptic action potentials. Furthermore, when the uIPSCs were blocked spontaneous PSCs could still be observed. We also studied uIPSCs evoked by multiple spikes during paired pulse and train stimulation. The baseline PPR was depressing (0.8 ± 0.2; n = 5) and, similarly, the response to train stimulation consisted of a constant depression with a facilitated response at the test pulse, consistent with previous findings (Planert et al., 2010). Interestingly, in both instances the paired pulse and train stimulation did not uncover a measurable uIPSC indicating a strong reduction of release probability by histamine. In summary, the results from the paired recording experiments suggest that histamine abolishes lateral inhibition between MSNs without affecting feedforward inhibition.
Discussion
The findings of the present study demonstrate that histamine dynamically modulates many aspects of the functional connectivity within the striatum. First, histamine suppresses both the cortical and thalamic excitatory drive to MSNs by acting at presynaptic H3 receptors. Second, histamine selectively modulates the dynamics of thalamostriatal, but not corticostriatal, synapses leading to a facilitation of the thalamic input. Thirdly, histamine abolishes lateral inhibition between MSNs without affecting feedforward inhibition mediated by FSIs onto MSNs. These findings suggest that when histaminergic neurons are active, such as during wakefulness and periods of increased attention, the striatum will have a facilitated response to thalamostriatal input and be dominated by feedforward inhibition.
Sparse innervation of the striatum
We observed a sparse innervation of the striatum by histamine-immunopositive fibers, consistent with previous findings (Takagi et al., 1986; Airaksinen and Panula, 1988). The sparse innervation, together with the fact that varicosities only infrequently make synapses (Takagi et al., 1986), raises the question of whether, and how, histamine could have widespread effects in the striatum. Although low affinity organic cation transporters might play a role in the uptake of histamine (Amphoux et al., 2006), to date no specific histamine transporter or uptake mechanism has been described in the brain. Thus, histamine is considered to be degraded in the extracellular space (Schwartz et al., 1991; Haas and Panula, 2003) with a half-life ranging in the tens of minutes (Schwartz et al., 1991). This suggests that histamine released by tonically active histaminergic neurons (Reiner and McGeer, 1987; Steininger et al., 1999; Takahashi et al., 2006) may diffuse from the site of release and affect large, if not all, areas of the striatum. The high expression of histamine receptors in the striatum (Hill and Young, 1980; Martinez-Mir et al., 1990; Vizuete et al., 1997; Pillot et al., 2002) supports the notion of a widespread effect of histamine, presumably through volume transmission.
Histaminergic modulation of excitatory inputs
The responses of both the direct and indirect pathway MSNs to excitatory cortical and thalamic drive are controlled by neuromodulators, local interneurons, as well as reciprocal connections between MSNs. All these factors will determine if, and when, action potentials are generated by the MSNs and will determine the subsequent downstream changes in the activity of basal ganglia output nuclei, basal ganglia targets and, ultimately, behavior.
We first set out to investigate whether histamine modulates activity at the principal excitatory afferents to MSNs, i.e., those derived from the cortex and thalamus. In all our experiments we used a single concentration of histamine (10 μm) which has been shown to be an effective concentration to study histamine in vitro (Brown and Haas, 1999; Atzori et al., 2000; Doreulee et al., 2001). However, it must be kept in mind that histamine concentrations in the intact brain might well be lower (Yoshitake et al., 2003; Chu et al., 2004). Deciding on the correct concentration is a general problem with in vitro preparations, as it is difficult to predict what the final concentration within the tissue will be. We therefore also studied the effect of lower concentrations of histamine (1 and 5 μm) on cortical excitatory transmission. The baseline synaptic responses and short-term dynamics were similar to those described previously (Ding et al., 2008; but see Smeal et al., 2007) and did not differ when either electrical or optical stimulation was used. We found that histamine negatively modulates both cortical and thalamic excitatory transmission at synapses on both classes of MSNs. Coapplication of the H3 receptor antagonist thioperamide and paired pulse experiments suggest that histamine is acting presynaptically at the H3 receptor, presumably through the negative modulation of Ca2+ inflow through voltage-activated Ca2+ channels (Brown and Haas, 1999), although a postsynaptic action, especially for corticostriatal transmission, cannot be excluded. Previous autoradiographic studies had already suggested high expression levels of this receptor in both the striatum and striatal afferents (Pillot et al., 2002). The H3 receptor is one of three G-protein coupled histamine receptors described in the brain and has been suggested to modulate transmission at many synapses (Haas and Panula, 2003). Interestingly, although suggested to have a high constitutive activity (Morisset et al., 2000) we did not observe a detectable increase in the amplitude of the excitatory (or inhibitory) postsynaptic responses after application of thioperamide by itself, suggesting low constitutive activity at these synapses (Threlfell et al., 2004). Ultimately, these results imply that stronger and/or more synchronous inputs from cortex and thalamus are necessary to initiate action potentials in MSNs during periods of histaminergic activity. Such negative modulation of excitatory inputs is reminiscent of gain control used by sensory systems (Petzold et al., 2009) to keep the postsynaptic response within a normal dynamic range and preventing input saturation.
However, trains of stimulation at corticostriatal and thalamostriatal synapses revealed that histamine selectively alters the short-term dynamics of thalamostriatal synapses, changing them from depressing to facilitating synapses (Thomson, 2000). Therefore, it seems that synchronous input from the thalamus is selectively facilitated in the presence of histamine and, compared with cortical input, is more likely to lead to action potential generation in MSNs. This fits well with the suggestion for the thalamic intralaminar nuclei having a general activating function (Kinomura et al., 1996) and a histaminergic system which is important for the maintenance of arousal and vigilance (Lin et al., 1988; Parmentier et al., 2002), but it might also facilitate the transmission of sensory information to the striatum (Matsumoto et al., 2001). Finally, the success of either cortical or thalamic excitatory input to elicit action potentials is dependent on the resting membrane potential of the MSNs. We found that MSNs are slightly depolarized by histamine acting at H2 receptors (Vizuete et al., 1997) most likely through activation of a subthreshold conductance (Haas and Panula, 2003).
Histamine differentially modulates striatal inhibition
The activity of striatal MSNs and their response to excitatory input, is further modulated by concurrent inhibition derived from collaterals of neighboring MSNs and local interneurons (Tepper and Plenz, 2006; Ponzi and Wickens, 2010). As a first test of the hypothesis that histamine modulates inhibitory input to MSNs we used intrastriatal electrical stimulation, in the presence of blockers of excitatory transmission, to recruit all inhibitory afferents to MSNs simultaneously. We observed a strong negative modulation of striatal inhibitory transmission at synapses on both classes of MSN, which was predominantly mediated through H3 receptors, although part of the modulation of the inhibitory response to D1 MSNs was through H2 receptors. This latter effect may be mediated through activation of striatal cholinergic interneurons as H2 receptor activation increases striatal acetylcholine release (Prast et al., 1999) and acetylcholine can modulate glutamatergic (Pakhotin and Bracci, 2007; Ding et al., 2010) and GABAergic transmission (Sugita et al., 1991; Koós and Tepper, 2002), although more complex interactions with other neuromodulatory pathways cannot be excluded (Threlfell and Cragg, 2011).
One might predict that the negative modulation of inhibitory currents by histamine reflects modulation of synapses located close to the soma i.e., those made by the FSIs onto MSNs (Tepper and Bolam, 2004). However, dual recordings of connected FSI–MSN pairs revealed that histamine did not affect this connection. This suggests that feedforward inhibition, which has been suggested to play a role in controlling spike timing and filtering of cortical input (Koós and Tepper, 1999; Mallet et al., 2005), is not affected by the presence of histamine. The second major inhibitory input to MSNs comes from reciprocal connections between MSNs (Tepper and Plenz, 2006). These synapses are made more distally on MSN dendrites (Somogyi et al., 1981; Bolam and Izzo, 1988) and are weaker than that of FSIs (Stern et al., 1998; Wilson, 2007; Planert et al., 2010). However, as they make up 95% of the total striatal neuron population, they could contribute substantially to the intrastriatal evoked inhibitory currents. This was confirmed by dual recordings of connected MSN–MSN pairs, which revealed that histamine abolishes the inhibitory connection between MSNs. Part of the reason why lateral inhibition is difficult to observe in vivo (Jaeger et al., 1994; Stern et al., 1998) might well be the persistent firing of histaminergic neurons under some anesthetic regimes (Reiner and McGeer, 1987). The precise role for lateral inhibition in striatal computation is still a matter of debate. It has been suggested to facilitate excitatory inputs by generating small depolarizations, mediate surround inhibition (although see Jaeger et al., 1994) or modulate dendritic processing of excitatory inputs (Carter and Sabatini, 2004; Tepper and Plenz, 2006; Wilson, 2007). Combined, these findings suggest that histamine modulates lateral inhibition between MSNs, but not feedforward inhibition mediated by FSIs, altering the response of the striatal microcircuit to excitatory inputs.
In conclusion, we suggest that histaminergic activity, during wakefulness and states of increased attention, entrains striatal information processing by differentially affecting the flow of excitatory inputs to the striatum and simultaneous intrastriatal processing of those inputs. Interestingly, recent studies have indicated a role for histaminergic neurotransmission in the mechanism and modulation of Tourette's syndrome (Ercan-Sencicek et al., 2010) and the effect of l-dopa treatment in Parkinson's disease (Yanovsky et al., 2011), suggesting histaminergic drugs might well be efficacious for these and other disorders involving the basal ganglia (Schwartz, 2011). Last, the widespread projections of the histaminergic system suggest that histamine might modulate information processing similarly in widespread regions of the brain.
Footnotes
This research was supported by the European Community (FP7: HEALTH-F2-2008-201716) and the Medical Research Council, UK (Grant U138164490). We thank K. Newton, K. Whitworth, C. Francis, G. Hazel, L. Norman, and B. Micklem for technical assistance. We thank L. Upton and W. Nissen for help setting up mouse surgery, D. Kaetzel and M. Kohl for advice on optogenetic stimulation, S. Threlfell for comments on a draft of this manuscript, and K.C. Nakamura for advice on immunolabeling for preproenkephalin. An abstract of this work has been awarded the Young Investigators Award by the European Histamine Research Society.
- Correspondence should be addressed to Tommas J. Ellender, MRC Anatomical Neuropharmacology Unit, Mansfield Road, OX1 3TH, Oxford, UK. tommas.ellender{at}pharm.ox.ac.uk