Differential Synaptic and Extrasynaptic Glutamate-Receptor Alterations in Striatal Medium-Sized Spiny Neurons of Aged YAC 128 Huntington ’ s Disease Mice

Huntington’s disease (HD) is a late-onset, slowly progressing neurodegenerative disorder caused by an expansion of glutamine repeats. The YAC128 mouse model has been widely used to study the progression of HD symptoms, but little is known about synaptic alterations in very old animals. The present experiments examined synaptic properties of striatal medium-sized spiny neurons (MSNs) in 16 month-old YAC128 mice. These mice were crossed with mice expressing enhanced green fluorescent protein (EGFP) under the control of either D1 or D2 dopamine receptor promoters to identify MSNs originating the direct and indirect pathways, respectively. The input-output curves of evoked excitatory postsynaptic currents mediated by activation of the ?-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid (AMPA) or N-methyl-D-aspartate (NMDA) receptors were reduced in MSNs in both pathways. In the presence of DL-threo-?-Benzyloxyaspartic acid (DL-TBOA), a glutamate transporter blocker used to increase activation of extrasynaptic receptors, NMDA receptor-mediated currents displayed altered amplitudes, longer decay times, and greater charge (response areas) in both direct and indirect pathway MSNs in YAC128 mice compared to wildtype controls. Amplitudes were significantly increased, primarily in direct pathway MSNs while normalized areas were significantly increased only in indirect pathway MSNs, suggesting that the two types of MSNs are affected in different ways. It may be that indirect pathway neurons are more susceptible to changes in glutamate transport. Taken together, the present findings demonstrate differential alterations in synaptic versus extrasynaptic NMDA receptors in both direct and indirect pathway MSNs in late HD, which may contribute to the dysfunction and degeneration in both pathways.


Introduction
Huntington's disease (HD), a slowly progressing neurodegenerative disorder caused by an expansion of glutamine (CAG) repeats, is characterized by motor, psychiatric and cognitive symptoms 1 .The YAC128 mouse model has been widely used to examine mechanisms of HD.YAC128 mice carry the entire human HD gene containing 128 CAG repeats on a yeast artificial chromosome (line 53) and express full-length human mutant huntingtin protein 2 .These mice display a hyperkinetic phenotype at 3 months of age, followed by motor deficits at 6 months, with eventual progression to hypokinesia by 12 months 3 .The behavioral changes are associated with biphasic alterations in excitatory synaptic transmission to striatal medium-sized spiny neurons (MSNs) of the direct (expressing dopamine D1 receptors) and indirect (expressing dopamine D2 receptors) striatal output pathways 4 , 5 .At the early, pre-symptomatic stage, glutamate transmission is increased in both direct and indirect pathways.In contrast, at 12 months of age, the more symptomatic phase, glutamatergic transmission is markedly reduced in direct pathway MSNs, while only a trend towards a reduction in glutamatergic inputs is observed in D2 MSNs 4 .Such biphasic alterations are also observed in evoked ?-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptor (AMPAR)-mediated currents, demonstrated by an increase in the peak amplitude in indirect pathway MSNs at 1.5 months and a reduction in direct pathway MSNs at 12 months 4 .Alterations in synaptic communication lead to a progressive disconnection between cortex and striatum and a loss of synaptic markets 21 .In these conditions, release of glutamate is more likely to activate extrasynaptic Nmethyl-D-aspartate receptors NMDARs), which are known to mediate apoptotic cascades 14 .Indeed, an increase in proapoptotic extrasynaptic NMDAR function occurs in YAC128 MSNs at the presymptomatic and symptomatic stages 6 .However, differences in extrasynaptic NMDARs from the direct and indirect pathways were not examined.This is important as studies have shown that MSNs of the indirect pathway are more vulnerable in HD 2 .
In the present study, we examined synaptic versus extrasynaptic electrophysiological changes induced by activation of AMPA

Introduction
Huntington's disease (HD), a slowly progressing neurodegenerative disorder caused by an expansion of glutamine (CAG) repeats, is characterized by motor, psychiatric and cognitive symptoms 1 .The YAC128 mouse model has been widely used to examine mechanisms of HD.YAC128 mice carry the entire human HD gene containing 128 CAG repeats on a yeast artificial chromosome (line 53) and express full-length human mutant huntingtin protein 2 .These mice display a hyperkinetic phenotype at 3 months of age, followed by motor deficits at 6 months, with eventual progression to hypokinesia by 12 months 3 .The behavioral changes are associated with biphasic alterations in excitatory synaptic transmission to striatal medium-sized spiny neurons (MSNs) of the direct (expressing dopamine D1 receptors) and indirect (expressing dopamine D2 receptors) striatal output pathways 4 , 5 .At the early, pre-symptomatic stage, glutamate transmission is increased in both direct and indirect pathways.In contrast, at 12 months of age, the more symptomatic phase, glutamatergic transmission is markedly reduced in direct pathway MSNs, while only a trend towards a reduction in glutamatergic inputs is observed in D2 MSNs 4 .Such biphasic alterations are also observed in evoked ?-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptor (AMPAR)-mediated currents, demonstrated by an increase in the peak amplitude in indirect pathway MSNs at 1.5 months and a reduction in direct pathway MSNs at 12 months 4 .Alterations in synaptic communication lead to a progressive disconnection between cortex and striatum and a loss of synaptic markets 21 .In these conditions, release of glutamate is more likely to activate extrasynaptic Nmethyl-D-aspartate receptors NMDARs), which are known to mediate apoptotic cascades 14 .Indeed, an increase in proapoptotic extrasynaptic NMDAR function occurs in YAC128 MSNs at the presymptomatic and symptomatic stages 6 .However, differences in extrasynaptic NMDARs from the direct and indirect pathways were not examined.This is important as studies have shown that MSNs of the indirect pathway are more vulnerable in HD 2 .
In the present study, we examined synaptic versus extrasynaptic electrophysiological changes induced by activation of AMPA

Introduction
Huntington's disease (HD), a slowly progressing neurodegenerative disorder caused by an expansion of glutamine (CAG) repeats, is characterized by motor, psychiatric and cognitive symptoms 1 .The YAC128 mouse model has been widely used to examine mechanisms of HD.YAC128 mice carry the entire human HD gene containing 128 CAG repeats on a yeast artificial chromosome (line 53) and express full-length human mutant huntingtin protein 2 .These mice display a hyperkinetic phenotype at 3 months of age, followed by motor deficits at 6 months, with eventual progression to hypokinesia by 12 months 3 .The behavioral changes are associated with biphasic alterations in excitatory synaptic transmission to striatal medium-sized spiny neurons (MSNs) of the direct (expressing dopamine D1 receptors) and indirect (expressing dopamine D2 receptors) striatal output pathways 4 , 5 .At the early, pre-symptomatic stage, glutamate transmission is increased in both direct and indirect pathways.In contrast, at 12 months of age, the more symptomatic phase, glutamatergic transmission is markedly reduced in direct pathway MSNs, while only a trend towards a reduction in glutamatergic inputs is observed in D2 MSNs 4 .Such biphasic alterations are also observed in evoked ?-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptor (AMPAR)-mediated currents, demonstrated by an increase in the peak amplitude in indirect pathway MSNs at 1.5 months and a reduction in direct pathway MSNs at 12 months 4 .Alterations in synaptic communication lead to a progressive disconnection between cortex and striatum and a loss of synaptic markets 21 .In these conditions, release of glutamate is more likely to activate extrasynaptic Nmethyl-D-aspartate receptors NMDARs), which are known to mediate apoptotic cascades 14 .Indeed, an increase in proapoptotic extrasynaptic NMDAR function occurs in YAC128 MSNs at the presymptomatic and symptomatic stages 6 .However, differences in extrasynaptic NMDARs from the direct and indirect pathways were not examined.This is important as studies have shown that MSNs of the indirect pathway are more vulnerable in HD 2 .
In the present study, we examined synaptic versus extrasynaptic electrophysiological changes induced by activation of AMPA and NMDA receptors in direct and indirect pathway MSNs of 16 month-old YAC128 mice and their age-matched wild type (WT) controls.Results revealed differential changes in synaptic and extrasynaptic activity of MSNs which could have important implications to understand the differential vulnerability of MSNs in these two striatal output pathways in HD.

Materials and Methods
All experimental procedures were performed in accordance with the United States Public Health Service Guide for Care and Use of Laboratory Animals and were approved by the Institutional Animal Care and Use Committee at the University of California, Los Angeles (UCLA).Experiments were conducted in WT and YAC128 mice crossbred to FVB/N mice expressing enhanced green fluorescent protein (EGFP) under the control of the D1 or D2 dopamine receptor promoter.All mice were obtained from our breeding colonies at UCLA.Each experimental or control group consisted of 5-10 mice.
After 1 h incubation, direct and indirect pathway MSNs were selected for recordings.Cells were visualized using a 40x waterimmersion lens on an Olympus microscope (BX50WI) equipped with differential interference contrast optics and fluorescence.After identifying MSNs with infrared videomicroscopy (QICAM-IR Fast 1394, Qimaging), the filter was switched to fluorescence to determine whether the cell was labeled with EGFP.The digitized infrared image was superimposed over the fluorescence image, and electrophysiological recordings proceeded only if the cell identified with infrared light overlapped with EGFP fluorescence.
All experiments were performed in voltage clamp mode, with patch electrodes (3-5 M?) filled with the following internal solution (in mM): 130 Cs-methanesulfonate, 10 CsCl, 4 NaCl, 1 MgCl 2 , 5 MgATP, 5 EGTA, 10 HEPES, 0.5 GTP, 10 phosphocreatine, (pH 7.25-7.3,osmolality, 280-290 mOsm).QX-314 (4 mM) was added to the intracellular solution to prevent Na + channel activation when stimulating or holding the membrane at depolarized potentials.Synaptic stimulation: To assess input-output functions, a monopolar glass electrode (impedance 1 M?) was placed in the corpus callosum 200-300 ?m from the MSN.To examine AMPAR-mediated currents, stimuli of increasing intensities (0.01-0.2 mA) were applied every 10 s, while for NMDAR-mediated currents stimuli were applied every 20 s.To record AMPAR-mediated currents, the membrane potential was clamped at -70mV in the presence of bicuculline (BIC, 10 ?M).NMDAR-mediated currents were recorded at a holding potential of +40 mV in the presence of BIC (10 ?M) and 6-Cyano-7nitroquinoxaline-2,3dione (CNQX, 10 ?M), which blocks AMPAR-mediated currents.Glycine (20 ?M) and strychnine (10 ?M) also were included to augment NMDAR function and block inhibitory glycine receptors, respectively 6 .DL-threo-?-Benzyloxyaspartic acid (DL-TBOA, 30 ?M), a blocker of excitatory amino acid transporters, also was used to promote spillover of glutamate from synaptic receptors onto extrasynaptic NMDARs 6 .At this concentration, the blocker has no direct effects on NMDARs 22 .For this experiment, the current intensity that evoked 75% of the peak amplitude response was used.Peak amplitude, area, and decay time were determined using ClampFit software.Decay times were assessed using the 90-10% portion of the decay phase, where 100% was the peak amplitude and 0% was at baseline.Thus, the decay time is the absolute time measurement of the decay phase of the response between 90% and 10% peak amplitude values.
Values in figures and text are means ± SEMs.Differences between group means were assessed with appropriate t-tests and two-way analyses of variance (ANOVA) with one repeated measure, followed by Bonferroni post hoc tests.Differences were considered statistically significant if p<0.05.

Results
Evoked excitatory currents were decreased in YAC128 direct and indirect pathway MSNs.

Materials and Methods
All experimental procedures were performed in accordance with the United States Public Health Service Guide for Care and Use of Laboratory Animals and were approved by the Institutional Animal Care and Use Committee at the University of California, Los Angeles (UCLA).Experiments were conducted in WT and YAC128 mice crossbred to FVB/N mice expressing enhanced green fluorescent protein (EGFP) under the control of the D1 or D2 dopamine receptor promoter.All mice were obtained from our breeding colonies at UCLA.Each experimental or control group consisted of 5-10 mice.
After 1 h incubation, direct and indirect pathway MSNs were selected for recordings.Cells were visualized using a 40x waterimmersion lens on an Olympus microscope (BX50WI) equipped with differential interference contrast optics and fluorescence.After identifying MSNs with infrared videomicroscopy (QICAM-IR Fast 1394, Qimaging), the filter was switched to fluorescence to determine whether the cell was labeled with EGFP.The digitized infrared image was superimposed over the fluorescence image, and electrophysiological recordings proceeded only if the cell identified with infrared light overlapped with EGFP fluorescence.
All experiments were performed in voltage clamp mode, with patch electrodes (3-5 M?) filled with the following internal solution (in mM): 130 Cs-methanesulfonate, 10 CsCl, 4 NaCl, 1 MgCl 2 , 5 MgATP, 5 EGTA, 10 HEPES, 0.5 GTP, 10 phosphocreatine, (pH 7.25-7.3,osmolality, 280-290 mOsm).QX-314 (4 mM) was added to the intracellular solution to prevent Na + channel activation when stimulating or holding the membrane at depolarized potentials.Synaptic stimulation: To assess input-output functions, a monopolar glass electrode (impedance 1 M?) was placed in the corpus callosum 200-300 ?m from the MSN.To examine AMPAR-mediated currents, stimuli of increasing intensities (0.01-0.2 mA) were applied every 10 s, while for NMDAR-mediated currents stimuli were applied every 20 s.To record AMPAR-mediated currents, the membrane potential was clamped at -70mV in the presence of bicuculline (BIC, 10 ?M).NMDAR-mediated currents were recorded at a holding potential of +40 mV in the presence of BIC (10 ?M) and 6-Cyano-7nitroquinoxaline-2,3dione (CNQX, 10 ?M), which blocks AMPAR-mediated currents.Glycine (20 ?M) and strychnine (10 ?M) also were included to augment NMDAR function and block inhibitory glycine receptors, respectively 6 .DL-threo-?-Benzyloxyaspartic acid (DL-TBOA, 30 ?M), a blocker of excitatory amino acid transporters, also was used to promote spillover of glutamate from synaptic receptors onto extrasynaptic NMDARs 6 .At this concentration, the blocker has no direct effects on NMDARs 22 .For this experiment, the current intensity that evoked 75% of the peak amplitude response was used.Peak amplitude, area, and decay time were determined using ClampFit software.Decay times were assessed using the 90-10% portion of the decay phase, where 100% was the peak amplitude and 0% was at baseline.Thus, the decay time is the absolute time measurement of the decay phase of the response between 90% and 10% peak amplitude values.
Values in figures and text are means ± SEMs.Differences between group means were assessed with appropriate t-tests and two-way analyses of variance (ANOVA) with one repeated measure, followed by Bonferroni post hoc tests.Differences were considered statistically significant if p<0.05.

Materials and Methods
All experimental procedures were performed in accordance with the United States Public Health Service Guide for Care and Use of Laboratory Animals and were approved by the Institutional Animal Care and Use Committee at the University of California, Los Angeles (UCLA).Experiments were conducted in WT and YAC128 mice crossbred to FVB/N mice expressing enhanced green fluorescent protein (EGFP) under the control of the D1 or D2 dopamine receptor promoter.All mice were obtained from our breeding colonies at UCLA.Each experimental or control group consisted of 5-10 mice.
After 1 h incubation, direct and indirect pathway MSNs were selected for recordings.Cells were visualized using a 40x waterimmersion lens on an Olympus microscope (BX50WI) equipped with differential interference contrast optics and fluorescence.After identifying MSNs with infrared videomicroscopy (QICAM-IR Fast 1394, Qimaging), the filter was switched to fluorescence to determine whether the cell was labeled with EGFP.The digitized infrared image was superimposed over the fluorescence image, and electrophysiological recordings proceeded only if the cell identified with infrared light overlapped with EGFP fluorescence.
All experiments were performed in voltage clamp mode, with patch electrodes (3-5 M?) filled with the following internal solution (in mM): 130 Cs-methanesulfonate, 10 CsCl, 4 NaCl, 1 MgCl 2 , 5 MgATP, 5 EGTA, 10 HEPES, 0.5 GTP, 10 phosphocreatine, (pH 7.25-7.3,osmolality, 280-290 mOsm).QX-314 (4 mM) was added to the intracellular solution to prevent Na + channel activation when stimulating or holding the membrane at depolarized potentials.Synaptic stimulation: To assess input-output functions, a monopolar glass electrode (impedance 1 M?) was placed in the corpus callosum 200-300 ?m from the MSN.To examine AMPAR-mediated currents, stimuli of increasing intensities (0.01-0.2 mA) were applied every 10 s, while for NMDAR-mediated currents stimuli were applied every 20 s.To record AMPAR-mediated currents, the membrane potential was clamped at -70mV in the presence of bicuculline (BIC, 10 ?M).NMDAR-mediated currents were recorded at a holding potential of +40 mV in the presence of BIC (10 ?M) and 6-Cyano-7nitroquinoxaline-2,3dione (CNQX, 10 ?M), which blocks AMPAR-mediated currents.Glycine (20 ?M) and strychnine (10 ?M) also were included to augment NMDAR function and block inhibitory glycine receptors, respectively 6 .DL-threo-?-Benzyloxyaspartic acid (DL-TBOA, 30 ?M), a blocker of excitatory amino acid transporters, also was used to promote spillover of glutamate from synaptic receptors onto extrasynaptic NMDARs 6 .At this concentration, the blocker has no direct effects on NMDARs 22 .For this experiment, the current intensity that evoked 75% of the peak amplitude response was used.Peak amplitude, area, and decay time were determined using ClampFit software.Decay times were assessed using the 90-10% portion of the decay phase, where 100% was the peak amplitude and 0% was at baseline.Thus, the decay time is the absolute time measurement of the decay phase of the response between 90% and 10% peak amplitude values.
Values in figures and text are means ± SEMs.Differences between group means were assessed with appropriate t-tests and two-way analyses of variance (ANOVA) with one repeated measure, followed by Bonferroni post hoc tests.Differences were considered statistically significant if p<0.05.
The post hoc analysis revealed a significant difference in the peak NMDAR-mediated currents at the 0.04 mA stimulation intensity (t=2.787,p=0.008) (Fig. 1D).There were no significant differences in peak AMPAR-or NMDAR-mediated currents between direct or indirect pathway MSNs from either WT or YAC128 mice.Furthermore, there were no differences in NMDA/AMPA ratios among direct and indirect pathway MSNs in WT and YAC128 mice (0.51±0.074 vs. 0.44±0.08 for WTs and YAC128 from direct pathway MSNs, respectively, p=0.542; 0.45±0.047vs. 0.56±0.056for WTs and YAC128 from indirect pathway MSNs, respectively, p=0.135).
The post hoc analysis revealed a significant difference in the peak NMDAR-mediated currents at the 0.04 mA stimulation intensity (t=2.787,p=0.008) (Fig. 1D).There were no significant differences in peak AMPAR-or NMDAR-mediated currents between direct or indirect pathway MSNs from either WT or YAC128 mice.Furthermore, there were no differences in NMDA/AMPA ratios among direct and indirect pathway MSNs in WT and YAC128 mice (0.51±0.074 vs. 0.44±0.08 for WTs and YAC128 from direct pathway MSNs, respectively, p=0.542; 0.45±0.047vs. 0.56±0.056for WTs and YAC128 from indirect pathway MSNs, respectively, p=0.135).
The post hoc analysis revealed a significant difference in the peak NMDAR-mediated currents at the 0.04 mA stimulation intensity (t=2.787,p=0.008) (Fig. 1D).There were no significant differences in peak AMPAR-or NMDAR-mediated currents between direct or indirect pathway MSNs from either WT or YAC128 mice.Furthermore, there were no differences in NMDA/AMPA ratios among direct and indirect pathway MSNs in WT and YAC128 mice (0.51±0.074 vs. 0.44±0.08 for WTs and YAC128 from direct pathway MSNs, respectively, p=0.542; 0.45±0.047vs. 0.56±0.056for WTs and YAC128 from indirect pathway MSNs, respectively, p=0.135).

Glutamate transport block revealed alterations in extrasynaptic NMDAR-mediated responses in YAC128 MSNs.
We used DL-TBOA (30 ?M), a glutamate transport blocker which promotes activation of extrasynaptic NMDARs through glutamate spillover, to assess differences in evoked NMDAR-mediated currents in direct and indirect pathway MSNs.We examined alterations in four indices, peak amplitude, decay time, response area and response area normalized by peak response separately for direct or indirect pathway MSNs (Fig. 2).An increase in the contribution from extrasynaptic NMDA receptors would be shown by changes in peak amplitude, decay time and response area of the currents.We only tested the effects of TBOA at the stimulus intensity that produced 75% of the maximum response for each neuron.In WTs for both direct and indirect pathway MSNs, peak amplitude decreased significantly in TBOA (t=2.177,p=0.047; t=2.684, p=0.016 for direct and indirect pathway MSNs, respectively) (Fig. 2B).In both direct and indirect pathway MSNs, almost all neurons (6/7 and 9/10 for direct and indirect pathway MSNs, respectively) showed a decrease in the peak response amplitude although for each group there was considerable variation in the absolute amplitudes of the responses of the neurons.In contrast, in direct pathway MSNs of YAC128 mice, peak amplitude increased significantly (t=4.128,p=0.001; 8/9 neurons) while in indirect pathway MSNs peak amplitude decreased significantly (t=6.017,p<0.001; 7/7 neurons) (Fig. 2B).
Because DL-TBOA affected direct and indirect pathway MSN peak values in opposing ways, the area was normalized by peak amplitude ((pA*ms)/pA) to verify a difference in the density of extrasynaptic NMDARs between direct and indirect pathway MSNs 6 .In this way the relative area could be compared without the confounding influence of the peak amplitude.Normalized response area increased significantly in all groups (t=5.090,p<0.001; t=2.64, p=0.017 for direct and indirect pathway MSNs in WTs, respectively; t=4.125, p=0.001; t=6.622, p<0.001 for direct and indirect pathway MSNs in YAC128, respectively) (Fig. 2E).In addition, the normalized area increase was significantly greater for indirect pathway MSNs in YAC128 mice compared to WTs (t=3.649,p=0.001).These findings indicate that both response amplitude and decay are affected by TBOA but in slightly different ways in direct and indirect pathway MSNs in YAC128 mice.To more specifically compare the effects of TBOA in direct and indirect pathway MSNs, changes induced by TBOA were converted to percentages (Fig. 3).In direct pathway MSNs, TBOA decreased the evoked NMDAR peak current in WTs but increased it in YAC128 mice (t=6.449,p<0.001) (Fig. 3A).In indirect pathway MSNs TBOA decreased the peak in both WT and We used DL-TBOA (30 ?M), a glutamate transport blocker which promotes activation of extrasynaptic NMDARs through glutamate spillover, to assess differences in evoked NMDAR-mediated currents in direct and indirect pathway MSNs.We examined alterations in four indices, peak amplitude, decay time, response area and response area normalized by peak response separately for direct or indirect pathway MSNs (Fig. 2).An increase in the contribution from extrasynaptic NMDA receptors would be shown by changes in peak amplitude, decay time and response area of the currents.We only tested the effects of TBOA at the stimulus intensity that produced 75% of the maximum response for each neuron.In WTs for both direct and indirect pathway MSNs, peak amplitude decreased significantly in TBOA (t=2.177,p=0.047; t=2.684, p=0.016 for direct and indirect pathway MSNs, respectively) (Fig. 2B).In both direct and indirect pathway MSNs, almost all neurons (6/7 and 9/10 for direct and indirect pathway MSNs, respectively) showed a decrease in the peak response amplitude although for each group there was considerable variation in the absolute amplitudes of the responses of the neurons.In contrast, in direct pathway MSNs of YAC128 mice, peak amplitude increased significantly (t=4.128,p=0.001; 8/9 neurons) while in indirect pathway MSNs peak amplitude decreased significantly (t=6.017,p<0.001; 7/7 neurons) (Fig. 2B).
Because DL-TBOA affected direct and indirect pathway MSN peak values in opposing ways, the area was normalized by peak amplitude ((pA*ms)/pA) to verify a difference in the density of extrasynaptic NMDARs between direct and indirect pathway MSNs 6 .In this way the relative area could be compared without the confounding influence of the peak amplitude.Normalized response area increased significantly in all groups (t=5.090,p<0.001; t=2.64, p=0.017 for direct and indirect pathway MSNs in WTs, respectively; t=4.125, p=0.001; t=6.622, p<0.001 for direct and indirect pathway MSNs in YAC128, respectively) (Fig. 2E).In addition, the normalized area increase was significantly greater for indirect pathway MSNs in YAC128 mice compared to WTs (t=3.649,p=0.001).These findings indicate that both response amplitude and decay are affected by TBOA but in slightly different ways in direct and indirect pathway MSNs in YAC128 mice.To more specifically compare the effects of TBOA in direct and indirect pathway MSNs, changes induced by TBOA were converted to percentages (Fig. 3).In direct pathway MSNs, TBOA decreased the evoked NMDAR peak current in WTs but increased it in YAC128 mice (t=6.449,p<0.001) (Fig. 3A).In indirect pathway MSNs TBOA decreased the peak in both WT and We used DL-TBOA (30 ?M), a glutamate transport blocker which promotes activation of extrasynaptic NMDARs through glutamate spillover, to assess differences in evoked NMDAR-mediated currents in direct and indirect pathway MSNs.We examined alterations in four indices, peak amplitude, decay time, response area and response area normalized by peak response separately for direct or indirect pathway MSNs (Fig. 2).An increase in the contribution from extrasynaptic NMDA receptors would be shown by changes in peak amplitude, decay time and response area of the currents.We only tested the effects of TBOA at the stimulus intensity that produced 75% of the maximum response for each neuron.In WTs for both direct and indirect pathway MSNs, peak amplitude decreased significantly in TBOA (t=2.177,p=0.047; t=2.684, p=0.016 for direct and indirect pathway MSNs, respectively) (Fig. 2B).In both direct and indirect pathway MSNs, almost all neurons (6/7 and 9/10 for direct and indirect pathway MSNs, respectively) showed a decrease in the peak response amplitude although for each group there was considerable variation in the absolute amplitudes of the responses of the neurons.In contrast, in direct pathway MSNs of YAC128 mice, peak amplitude increased significantly (t=4.128,p=0.001; 8/9 neurons) while in indirect pathway MSNs peak amplitude decreased significantly (t=6.017,p<0.001; 7/7 neurons) (Fig. 2B).
Because DL-TBOA affected direct and indirect pathway MSN peak values in opposing ways, the area was normalized by peak amplitude ((pA*ms)/pA) to verify a difference in the density of extrasynaptic NMDARs between direct and indirect pathway MSNs 6 .In this way the relative area could be compared without the confounding influence of the peak amplitude.Normalized response area increased significantly in all groups (t=5.090,p<0.001; t=2.64, p=0.017 for direct and indirect pathway MSNs in WTs, respectively; t=4.125, p=0.001; t=6.622, p<0.001 for direct and indirect pathway MSNs in YAC128, respectively) (Fig. 2E).In addition, the normalized area increase was significantly greater for indirect pathway MSNs in YAC128 mice compared to WTs (t=3.649,p=0.001).These findings indicate that both response amplitude and decay are affected by TBOA but in slightly different ways in direct and indirect pathway MSNs in YAC128 mice.To more specifically compare the effects of TBOA in direct and indirect pathway MSNs, changes induced by TBOA were converted to percentages (Fig. 3).In direct pathway MSNs, TBOA decreased the evoked NMDAR peak current in WTs but increased it in YAC128 mice (t=6.449,p<0.001) (Fig. 3A).In indirect pathway MSNs TBOA decreased the peak in both WT and YAC128 mice, but the reduction was significantly larger in YAC128 D2 MSNs (t=3.323,p=0.002) (Fig. 3A).The difference in peak amplitude between direct and indirect pathway MSNs in YAC128 mice also was significant (t=9.150,p<0.001).Decay time was significantly elevated in indirect YAC128 MSNs compared to WTs (t=3.601,p=0.001) (Fig. 3B) and also was significantly greater in indirect pathway MSNs compared to direct pathway MSNs in YAC128 mice (t=2.258,p=0.031).Area was significantly larger in YAC128 direct pathway MSNs compared to area of WTs (t=3.482,p=0.002) (Fig. 3C).The increased area of indirect pathway MSNs approached statistical significance (t=1.829,p=0.077).The increased area of direct versus indirect pathway MSNs was significantly greater in only the YAC128 mice (t=2.353,p<0.025).There was a significant increase in relative area in indirect pathway MSNs in YAC128 mice compared to WTs (t=5.012,p<0.001) as well as a significant increase in indirect pathway MSNs compared to direct pathway MSNs but only in MSNs in YAC128 mice (t=4.158,p<0.001) (Fig. 3D).

Discussion
The present study demonstrated decreases in evoked excitatory postsynaptic currents mediated by AMPARs and NMDARs in YAC128 direct and indirect pathway MSNs.Furthermore, in contrast to the downregulation of synaptic activity, NMDARmediated responses evoked in the presence of TBOA were increased in both direct and indirect pathway MSNs of YAC128 mice, but in slightly different ways.In direct pathway MSNs, response increases were mainly due to higher amplitudes while in indirect pathway MSNs, the increase was due to longer decay times.This outcome indicates differential changes in synaptic versus extrasynaptic NMDA receptors in both direct and indirect pathway MSNs from these older, symptomatic YAC128 mice.
We previously reported a progressive disconnection of striatal MSNs from their glutamatergic inputs in various models of HD 7 , 8 .In 12 month-old YAC128 mice we also showed that the reduction in the spontaneous excitatory postsynaptic current frequency was greater in direct than indirect pathway MSNs but we did not examine AMPAR and NMDAR responses separately and our results were based on AMPAR-mediated responses 4 .The reduction in evoked synaptic responses agrees with previous studies showing decreases in glutamate release as well as AMPAR-and NMDAR-mediated currents in symptomatic YAC128 mice 9 .The reduction in the amplitude of evoked responses indicates that there is a loss of glutamatergic inputs onto MSNs in YAC128 mice at this age for MSNs originating both pathways in HD.The loss of glutamatergic inputs may be due to pre-and postsynaptic mechanisms.In YAC128 mice a reduction in spine density has been observed 10 .While the reduction in spine density could be caused by pre-and post-synaptic mechanisms, recent studies demonstrate a critical role of postsynaptic NMDA receptors containing GluN3A subunits in HD spine loss 11 .
In contrast to the reduction in evoked synaptic currents, NMDA responses evoked in the presence of TBOA were increased.Previous studies demonstrated an increase in the extrasynaptic NMDAR-mediated responses in young YAC128 mice 6 .However, differences between direct and indirect pathway MSNs were not examined.The present study not only confirms that this increase in extrasynaptic NMDAR-mediated responses occurs in old YAC128 mice, but also demonstrates that it occurs in both direct and indirect pathway MSNs though it appears to be mechanistically due to differing underlying effetcs.Direct pathway MSNs show a larger increase in peak amplitude while indirect pathway MSNs display a larger increase in normalized area due to a longer decay time.This latter effect could suggest that MSNs of the indirect pathway are more sensitive to changes in glutamate transport, thus contributing to their increased vulnerability in HD.
NMDARs are composed by GluN2A and GluN2B subunits.GluN2A subunits are thought to be restricted mainly to the synaptic site 12 , while the GluN2B subunits are located on synaptic and extrasynaptic sites 13 .It has been suggested that the activation of the synaptic NMDARs is neuroprotective, while activation of extrasynaptic NMDA receptors stimulates a pro-apoptotic cellular pathway 14 .Alterations in NMDAR subunit trafficking is thought to contribute to increased density of GluN2B subunits at extrasynaptic sites in HD 15 , 16 .In a recent study employing co-culture of cortical and striatal MSNs from YAC128 mice, a larger extrasynaptic NMDAR-mediated current occurred in association with an increase in GluN2B subunit expression at the cellular surface compared with the co-culture obtained from WT mice 6 , 17 .In addition, low-dose memantine, a blocker of GluN2Bcontaining NMDARs at extrasynaptic sites, ameliorates neuropathological and behavioral manifestations of HD in YAC128 mice 6 , 18 YAC128 mice, but the reduction was significantly larger in YAC128 D2 MSNs (t=3.323,p=0.002) (Fig. 3A).The difference in peak amplitude between direct and indirect pathway MSNs in YAC128 mice also was significant (t=9.150,p<0.001).Decay time was significantly elevated in indirect YAC128 MSNs compared to WTs (t=3.601,p=0.001) (Fig. 3B) and also was significantly greater in indirect pathway MSNs compared to direct pathway MSNs in YAC128 mice (t=2.258,p=0.031).Area was significantly larger in YAC128 direct pathway MSNs compared to area of WTs (t=3.482,p=0.002) (Fig. 3C).The increased area of indirect pathway MSNs approached statistical significance (t=1.829,p=0.077).The increased area of direct versus indirect pathway MSNs was significantly greater in only the YAC128 mice (t=2.353,p<0.025).There was a significant increase in relative area in indirect pathway MSNs in YAC128 mice compared to WTs (t=5.012,p<0.001) as well as a significant increase in indirect pathway MSNs compared to direct pathway MSNs but only in MSNs in YAC128 mice (t=4.158,p<0.001) (Fig. 3D).

Discussion
The present study demonstrated decreases in evoked excitatory postsynaptic currents mediated by AMPARs and NMDARs in YAC128 direct and indirect pathway MSNs.Furthermore, in contrast to the downregulation of synaptic activity, NMDARmediated responses evoked in the presence of TBOA were increased in both direct and indirect pathway MSNs of YAC128 mice, but in slightly different ways.In direct pathway MSNs, response increases were mainly due to higher amplitudes while in indirect pathway MSNs, the increase was due to longer decay times.This outcome indicates differential changes in synaptic versus extrasynaptic NMDA receptors in both direct and indirect pathway MSNs from these older, symptomatic YAC128 mice.
We previously reported a progressive disconnection of striatal MSNs from their glutamatergic inputs in various models of HD 7 , 8 .In 12 month-old YAC128 mice we also showed that the reduction in the spontaneous excitatory postsynaptic current frequency was greater in direct than indirect pathway MSNs but we did not examine AMPAR and NMDAR responses separately and our results were based on AMPAR-mediated responses 4 .The reduction in evoked synaptic responses agrees with previous studies showing decreases in glutamate release as well as AMPAR-and NMDAR-mediated currents in symptomatic YAC128 mice 9 .The reduction in the amplitude of evoked responses indicates that there is a loss of glutamatergic inputs onto MSNs in YAC128 mice at this age for MSNs originating both pathways in HD.The loss of glutamatergic inputs may be due to pre-and postsynaptic mechanisms.In YAC128 mice a reduction in spine density has been observed 10 .While the reduction in spine density could be caused by pre-and post-synaptic mechanisms, recent studies demonstrate a critical role of postsynaptic NMDA receptors containing GluN3A subunits in HD spine loss 11 .
In contrast to the reduction in evoked synaptic currents, NMDA responses evoked in the presence of TBOA were increased.Previous studies demonstrated an increase in the extrasynaptic NMDAR-mediated responses in young YAC128 mice 6 .However, differences between direct and indirect pathway MSNs were not examined.The present study not only confirms that this increase in extrasynaptic NMDAR-mediated responses occurs in old YAC128 mice, but also demonstrates that it occurs in both direct and indirect pathway MSNs though it appears to be mechanistically due to differing underlying effetcs.Direct pathway MSNs show a larger increase in peak amplitude while indirect pathway MSNs display a larger increase in normalized area due to a longer decay time.This latter effect could suggest that MSNs of the indirect pathway are more sensitive to changes in glutamate transport, thus contributing to their increased vulnerability in HD.
NMDARs are composed by GluN2A and GluN2B subunits.GluN2A subunits are thought to be restricted mainly to the synaptic site 12 , while the GluN2B subunits are located on synaptic and extrasynaptic sites 13 .It has been suggested that the activation of the synaptic NMDARs is neuroprotective, while activation of extrasynaptic NMDA receptors stimulates a pro-apoptotic cellular pathway 14 .Alterations in NMDAR subunit trafficking is thought to contribute to increased density of GluN2B subunits at extrasynaptic sites in HD 15 , 16 .In a recent study employing co-culture of cortical and striatal MSNs from YAC128 mice, a larger extrasynaptic NMDAR-mediated current occurred in association with an increase in GluN2B subunit expression at the cellular surface compared with the co-culture obtained from WT mice 6 , 17 .In addition, low-dose memantine, a blocker of GluN2Bcontaining NMDARs at extrasynaptic sites, ameliorates neuropathological and behavioral manifestations of HD in YAC128 mice 6 , 18 YAC128 mice, but the reduction was significantly larger in YAC128 D2 MSNs (t=3.323,p=0.002) (Fig. 3A).The difference in peak amplitude between direct and indirect pathway MSNs in YAC128 mice also was significant (t=9.150,p<0.001).Decay time was significantly elevated in indirect YAC128 MSNs compared to WTs (t=3.601,p=0.001) (Fig. 3B) and also was significantly greater in indirect pathway MSNs compared to direct pathway MSNs in YAC128 mice (t=2.258,p=0.031).Area was significantly larger in YAC128 direct pathway MSNs compared to area of WTs (t=3.482,p=0.002) (Fig. 3C).The increased area of indirect pathway MSNs approached statistical significance (t=1.829,p=0.077).The increased area of direct versus indirect pathway MSNs was significantly greater in only the YAC128 mice (t=2.353,p<0.025).There was a significant increase in relative area in indirect pathway MSNs in YAC128 mice compared to WTs (t=5.012,p<0.001) as well as a significant increase in indirect pathway MSNs compared to direct pathway MSNs but only in MSNs in YAC128 mice (t=4.158,p<0.001) (Fig. 3D).

Discussion
The present study demonstrated decreases in evoked excitatory postsynaptic currents mediated by AMPARs and NMDARs in YAC128 direct and indirect pathway MSNs.Furthermore, in contrast to the downregulation of synaptic activity, NMDARmediated responses evoked in the presence of TBOA were increased in both direct and indirect pathway MSNs of YAC128 mice, but in slightly different ways.In direct pathway MSNs, response increases were mainly due to higher amplitudes while in indirect pathway MSNs, the increase was due to longer decay times.This outcome indicates differential changes in synaptic versus extrasynaptic NMDA receptors in both direct and indirect pathway MSNs from these older, symptomatic YAC128 mice.
We previously reported a progressive disconnection of striatal MSNs from their glutamatergic inputs in various models of HD 7 , 8 .In 12 month-old YAC128 mice we also showed that the reduction in the spontaneous excitatory postsynaptic current frequency was greater in direct than indirect pathway MSNs but we did not examine AMPAR and NMDAR responses separately and our results were based on AMPAR-mediated responses 4 .The reduction in evoked synaptic responses agrees with previous studies showing decreases in glutamate release as well as AMPAR-and NMDAR-mediated currents in symptomatic YAC128 mice 9 .The reduction in the amplitude of evoked responses indicates that there is a loss of glutamatergic inputs onto MSNs in YAC128 mice at this age for MSNs originating both pathways in HD.The loss of glutamatergic inputs may be due to pre-and postsynaptic mechanisms.In YAC128 mice a reduction in spine density has been observed 10 .While the reduction in spine density could be caused by pre-and post-synaptic mechanisms, recent studies demonstrate a critical role of postsynaptic NMDA receptors containing GluN3A subunits in HD spine loss 11 .
In contrast to the reduction in evoked synaptic currents, NMDA responses evoked in the presence of TBOA were increased.Previous studies demonstrated an increase in the extrasynaptic NMDAR-mediated responses in young YAC128 mice 6 .However, differences between direct and indirect pathway MSNs were not examined.The present study not only confirms that this increase in extrasynaptic NMDAR-mediated responses occurs in old YAC128 mice, but also demonstrates that it occurs in both direct and indirect pathway MSNs though it appears to be mechanistically due to differing underlying effetcs.Direct pathway MSNs show a larger increase in peak amplitude while indirect pathway MSNs display a larger increase in normalized area due to a longer decay time.This latter effect could suggest that MSNs of the indirect pathway are more sensitive to changes in glutamate transport, thus contributing to their increased vulnerability in HD.
NMDARs are composed by GluN2A and GluN2B subunits.GluN2A subunits are thought to be restricted mainly to the synaptic site 12 , while the GluN2B subunits are located on synaptic and extrasynaptic sites 13 .It has been suggested that the activation of the synaptic NMDARs is neuroprotective, while activation of extrasynaptic NMDA receptors stimulates a pro-apoptotic cellular pathway 14 .Alterations in NMDAR subunit trafficking is thought to contribute to increased density of GluN2B subunits at extrasynaptic sites in HD 15 , 16 .In a recent study employing co-culture of cortical and striatal MSNs from YAC128 mice, a larger extrasynaptic NMDAR-mediated current occurred in association with an increase in GluN2B subunit expression at the cellular surface compared with the co-culture obtained from WT mice 6 , 17 .In addition, low-dose memantine, a blocker of GluN2Bcontaining NMDARs at extrasynaptic sites, ameliorates neuropathological and behavioral manifestations of HD in YAC128 mice 6 , 18 . In co-cultured YAC128 MSNs, low doses of memantine and ifenprodil attenuated extrasynaptic NMDAR-mediated neuronal apoptosis 17 .
In conclusion, the present results showed that the glutamatergic inputs to MSNs are decreased in 16-month old YAC128 mice.This study also demonstrates that in late stage HD, NMDA responses evoked in both direct and indirect pathway MSNs in the presence of TBOA are significantly increased in YAC128 mice and the parameters for the increase are different.Direct pathway MSNs in YAC128 mice display increases in peak amplitude while indirect pathway MSNs in YAC128 mice display increases in normalized area due to significantly slower decay times.These results suggest that alterations in glutamate reuptake have different effects on indirect compared with direct pathway MSNs and highlight previous studies showing that MSNs of both pathways are differentially affected in mouse models of HD 19 , 20 .
In conclusion, the present results showed that the glutamatergic inputs to MSNs are decreased in 16-month old YAC128 mice.This study also demonstrates that in late stage HD, NMDA responses evoked in both direct and indirect pathway MSNs in the presence of TBOA are significantly increased in YAC128 mice and the parameters for the increase are different.Direct pathway MSNs in YAC128 mice display increases in peak amplitude while indirect pathway MSNs in YAC128 mice display increases in normalized area due to significantly slower decay times.These results suggest that alterations in glutamate reuptake have different effects on indirect compared with direct pathway MSNs and highlight previous studies showing that MSNs of both pathways are differentially affected in mouse models of HD 19 , 20 .
In conclusion, the present results showed that the glutamatergic inputs to MSNs are decreased in 16-month old YAC128 mice.This study also demonstrates that in late stage HD, NMDA responses evoked in both direct and indirect pathway MSNs in the presence of TBOA are significantly increased in YAC128 mice and the parameters for the increase are different.Direct pathway MSNs in YAC128 mice display increases in peak amplitude while indirect pathway MSNs in YAC128 mice display increases in normalized area due to significantly slower decay times.These results suggest that alterations in glutamate reuptake have different effects on indirect compared with direct pathway MSNs and highlight previous studies showing that MSNs of both pathways are differentially affected in mouse models of HD 19 , 20 .

Fig. 1 :
Fig. 1: AMPAR-and NMDAR-mediated currents were significantly reduced in direct and indirect pathway MSNs in YAC128 mice.A: Typical traces of AMPAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at the 0.10 mA stimulus intensity are shown.B: Input-output functions of evoked AMPAR-mediated currents were significantly decreased in both direct and indirect pathway MSNs of YAC128 mice.C: Typical traces of NMDAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at 0.10 mA stimulus intensity are shown.D: Input-output functions of evoked NMDAR-mediated currents also were significantly reduced in both direct and indirect pathway MSNs from YAC128 mice.In this and other figures * indicates p<0.05, ** indicates p<0.01, *** indicates p<0.001.See text for details of statistics.

Fig. 1 :
Fig. 1: AMPAR-and NMDAR-mediated currents were significantly reduced in direct and indirect pathway MSNs in YAC128 mice.A: Typical traces of AMPAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at the 0.10 mA stimulus intensity are shown.B: Input-output functions of evoked AMPAR-mediated currents were significantly decreased in both direct and indirect pathway MSNs of YAC128 mice.C: Typical traces of NMDAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at 0.10 mA stimulus intensity are shown.D: Input-output functions of evoked NMDAR-mediated currents also were significantly reduced in both direct and indirect pathway MSNs from YAC128 mice.In this and other figures * indicates p<0.05, ** indicates p<0.01, *** indicates p<0.001.See text for details of statistics.

Fig. 1 :
Fig. 1: AMPAR-and NMDAR-mediated currents were significantly reduced in direct and indirect pathway MSNs in YAC128 mice.A: Typical traces of AMPAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at the 0.10 mA stimulus intensity are shown.B: Input-output functions of evoked AMPAR-mediated currents were significantly decreased in both direct and indirect pathway MSNs of YAC128 mice.C: Typical traces of NMDAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at 0.10 mA stimulus intensity are shown.D: Input-output functions of evoked NMDAR-mediated currents also were significantly reduced in both direct and indirect pathway MSNs from YAC128 mice.In this and other figures * indicates p<0.05, ** indicates p<0.01, *** indicates p<0.001.See text for details of statistics.

Fig. 2 :
Fig. 2: DL-TBOA alters peak amplitude, decay, area and relative area of direct and indirect pathway MSNs of WT and YAC128 mice.A: Typical traces of NMDAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at 75% of the maximal stimulus intensity showing alterations in peak amplitudes and decay times.B: Peak amplitude is differentially altered in direct and indirect pathway MSNs by DL-TBOA.Peak amplitude increases in direct pathway MSNs but decreases in indirect pathway MSNs in YAC128 mice.C: In DL-TBOA response decay time increases in direct and indirect pathway MSNs in both WT and YAC128 mice.D: In DL-TBOA, response area increases only in direct pathway MSNs in YAC128 mice and in indirect pathway MSNs in both WT and YAC128 mice.E: In DL-TBOA, normalized area increases in all groups but displays the greatest increase in indirect pathway MSNs in YAC128 mice.

Fig. 2 :
Fig. 2: DL-TBOA alters peak amplitude, decay, area and relative area of direct and indirect pathway MSNs of WT and YAC128 mice.A: Typical traces of NMDAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at 75% of the maximal stimulus intensity showing alterations in peak amplitudes and decay times.B: Peak amplitude is differentially altered in direct and indirect pathway MSNs by DL-TBOA.Peak amplitude increases in direct pathway MSNs but decreases in indirect pathway MSNs in YAC128 mice.C: In DL-TBOA response decay time increases in direct and indirect pathway MSNs in both WT and YAC128 mice.D: In DL-TBOA, response area increases only in direct pathway MSNs in YAC128 mice and in indirect pathway MSNs in both WT and YAC128 mice.E: In DL-TBOA, normalized area increases in all groups but displays the greatest increase in indirect pathway MSNs in YAC128 mice.

Fig. 2 :
Fig. 2: DL-TBOA alters peak amplitude, decay, area and relative area of direct and indirect pathway MSNs of WT and YAC128 mice.A: Typical traces of NMDAR-mediated currents in WT and YAC128 direct and indirect pathway MSNs evoked at 75% of the maximal stimulus intensity showing alterations in peak amplitudes and decay times.B: Peak amplitude is differentially altered in direct and indirect pathway MSNs by DL-TBOA.Peak amplitude increases in direct pathway MSNs but decreases in indirect pathway MSNs in YAC128 mice.C: In DL-TBOA response decay time increases in direct and indirect pathway MSNs in both WT and YAC128 mice.D: In DL-TBOA, response area increases only in direct pathway MSNs in YAC128 mice and in indirect pathway MSNs in both WT and YAC128 mice.E: In DL-TBOA, normalized area increases in all groups but displays the greatest increase in indirect pathway MSNs in YAC128 mice.

Fig. 3 :
Fig. 3: Differential effects of DL-TBOA on direct and indirect pathway MSNs exemplified by percentage changes.A: Percentage changes in peak response amplitude were differentially altered in direct and indirect pathway MSNs of YAC128 mice.B: Percentage changes in decay times were greater in indirect pathway compared to direct pathway MSNs from YAC128 mice.C: Percentage change in response area were greatest in direct pathway MSNs of YAC128 mice.D: Normalized area increases were greatest in indirect pathway MSNs of YAC128 mice.

Fig. 3 :
Fig. 3: Differential effects of DL-TBOA on direct and indirect pathway MSNs exemplified by percentage changes.A: Percentage changes in peak response amplitude were differentially altered in direct and indirect pathway MSNs of YAC128 mice.B: Percentage changes in decay times were greater in indirect pathway compared to direct pathway MSNs from YAC128 mice.C: Percentage change in response area were greatest in direct pathway MSNs of YAC128 mice.D: Normalized area increases were greatest in indirect pathway MSNs of YAC128 mice.

Fig. 3 :
Fig. 3: Differential effects of DL-TBOA on direct and indirect pathway MSNs exemplified by percentage changes.A: Percentage changes in peak response amplitude were differentially altered in direct and indirect pathway MSNs of YAC128 mice.B: Percentage changes in decay times were greater in indirect pathway compared to direct pathway MSNs from YAC128 mice.C: Percentage change in response area were greatest in direct pathway MSNs of YAC128 mice.D: Normalized area increases were greatest in indirect pathway MSNs of YAC128 mice.