Glutamatergic dysfunction is strongly implicated in schizophrenia and mood disorders. GluA1 knockout (KO) mice display schizophrenia- and depression-related abnormalities. Here, we asked whether GluA1 KO show mania-related abnormalities. KO were tested for behavior in approach/avoid conflict tests, responses to repeated forced swim exposure, and locomotor responses under stress and after psychostimulant treatment. The effects of rapid dopamine depletion and treatment with lithium or a GSK-3β inhibitor (SB216763) on KO locomotor hyperactivity were tested. Results showed that KO exhibited novelty- and stress-induced locomotor hyperactivity, reduced forced swim immobility and alterations in approach/avoid conflict tests. Psychostimulant treatment and dopamine depletion exacerbated KO locomotor hyperactivity. Lithium, but not SB216763, treatment normalized KO anxiety-related behavior and partially reversed hyperlocomotor behavior, and also reversed elevated prefrontal cortex levels of phospho-MARCKS and phospho-neuromodulin. Collectively, these findings demonstrate mania-related abnormalities in GluA1 KO and, combined with previous findings, suggest this mutant may provide a novel model of features of schizoaffective disorder.
Glutamatergic dysfunction is strongly implicated in schizophrenia and mood disorders. GluA1 knockout (KO) mice display schizophrenia- and depression-related abnormalities. Here, we asked whether GluA1 KO show mania-related abnormalities. KO were tested for behavior in approach/avoid conflict tests, responses to repeated forced swim exposure, and locomotor responses under stress and after psychostimulant treatment. The effects of rapid dopamine depletion and treatment with lithium or a GSK-3β inhibitor (SB216763) on KO locomotor hyperactivity were tested. Results showed that KO exhibited novelty- and stress-induced locomotor hyperactivity, reduced forced swim immobility and alterations in approach/avoid conflict tests. Psychostimulant treatment and dopamine depletion exacerbated KO locomotor hyperactivity. Lithium, but not SB216763, treatment normalized KO anxiety-related behavior and partially reversed hyperlocomotor behavior, and also reversed elevated prefrontal cortex levels of phospho-MARCKS and phospho-neuromodulin. Collectively, these findings demonstrate mania-related abnormalities in GluA1 KO and, combined with previous findings, suggest this mutant may provide a novel model of features of schizoaffective disorder.
Genes and molecules involved in excitatory synapse function are attractive
candidates as risk factors for psychiatric conditions with a broad clinical
phenotype such as schizoaffective disorder. Such ‘synaptologies’
have been posited to underlie neurodevelopmental disorders such as autism (Sudhof, 2008) but could also contribute to the
pathophysiology of neuropsychiatric disorders with a major developmental component
such as schizoaffective disorder. In this context, L-glutamate is the major
excitatory neurotransmitter system in the central nervous system and a key regulator
of synaptic function and plasticity (Malenka and
Bear, 2004). Glutamatergic dysfunction is strongly implicated in
schizophrenia and mood disorders (Coyle,
2006).Glutamatergic neurotransmission is mediated by an array of receptors
belonging to the ionotropic (α-amino-3-hydroxy-5-methyl-4isoxazole
propionate [AMPAR], N-methyl-D-aspartate
[NMDAR], kainate) and metabotropic receptor (mGluR) subfamilies.
AMPAR are postsynaptic heteromeric proteins composed of one or more glutamate
receptor GluA1-GluA4 subunits (Shi et al.,
2001). The GluA1/2 heteromer, and coupling to its downstream
intracellular signaling pathways, is altered in rodents by treatment with anti-manic
drugs (e.g., lithium, valproate) and mania-inducing manipulations (e.g.,
psychostimulant treatment) (Du et al., 2008;
Du et al., 2007). There are also reports
of reduced GluA1 gene expression in the post-mortem brains of persons with bipolar
disorder (Beneyto et al., 2007).Important insight into the potential role of the GluA1 subtype has come from
studies in mutant mice with targeted deletion of GluA1 (GluA1
‘knockout,’ KO). For example, we recently reported that GluA1 KO
caused multiple behavioral abnormalities considered relevant to schizophrenia (Wiedholz et al., 2008). Interestingly, we and
others have also found that GluA1 KO exhibit disturbances on tests for emotionality
(Bannerman et al., 2004; Mead et al., 2006; Vekovischeva et al., 2004), and develop a
‘depression-related’ phenotype on various tests that entail repeated
exposure to stressful situations (Chourbaji et al.,
2008). The pleiotropic nature of genetic deletion of GluA1 suggests that
the phenotype of these mutants may more closely model features of more than one
neuropsychiatric disorder rather than any one major affective or psychotic condition
alone.There is an increasing view that despite their diagnostic demarcation,
certain forms of severe psychotic and mood disorders have a common
pathophysiological basis (Owen et al., 2007).
This is supported by the observation that the prevalence of schizophrenia and
bipolar disorder tends to cluster in families and share a genetic component (Cardno et al., 2002; Kendler et al., 1998; Owen et al., 2007; Park et al.,
2004; Potash et al., 2003). It has
also recently been shown that bipolar disorder and major depressive disorder share a
genetic susceptibility locus (McMahon et al., 2010). Clinically, individuals who
exhibit ‘illness during which there is a major depressive, manic, or mixed
episode concurrent with symptoms that meet criterion [A] for
schizophrenia’ meet diagnostic criteria for schizoaffective disorder (DSM-IV, 1994). However, the specific genetic
and molecular factors that put an individual at risk for schizoaffective disorder,
rather than a more discrete psychotic or depressive disorder, are not well
understood.Given previous studies have found that GluA1 KO mice exhibit schizophrenia-
and depression-related abnormalities, the aim of the present study was to evaluate
these mutants for other features of schizoaffective disorder with a focus on the
manic component. Mania is characterized by hyperactivity of movement and thought,
and can be precipitated or exacerbated by stress (Ambelas, 1979; Malkoff-Schwartz et al.,
2000). We assayed GluA1 KO mice for locomotor responses to novelty and
stress in an open field and behavioral responses to novel and repeated forced swim.
Because the manic component is also associated with increased self-esteem,
risk-taking and novelty-seeking, we tested the mutants for anxiety-related and
novelty-seeking behaviors in various tasks that differentially test these two drives
(elevated plus- and zero-maze, light/dark emergence test, stress-induced
hyperthermia).We went on to explore potential neurobiological mechanisms underlying
behavioral abnormalities in GluA1 KO. We tested whether the KO phenotype was rescued
by two drugs with known or hypothesized efficacy in bipolar disorder or
schizophrenia, lithium and the glycogen synthase kinase-3 beta inhibitor, SB216763.
Moreover, given our earlier finding that these KO mice had impaired striatal
dopamine clearance (Wiedholz et al., 2008),
we tested whether the hyperlocomotor phenotype was rescued by depletion of brain
dopamine. To identify molecular mechanisms associated with the GluA1 KO phenotype
and its predicted rescue by lithium, we evaluated the activity of two markers
(MARCKS and neuromodulin) of protein kinase C (PKC), an intracellular pathway
implicated in mania (Szabo et al., 2009).
Materials and Methods
Subjects
GluA1 KO were generated as previously described (Zamanillo et al., 1999) on a
129S1/Sv-p+Tyr+Kitl−/+
× 129X1/SvJ background. We have previously found these mice to be normal
on a range of simple measures of physical health, neurological and sensory
functions (Wiedholz et al., 2008) (Table 1; male WT=8, female
WT=6, male KO=8, female KO=6; counts by experimental
group (n) in legend), and motor coordination (Palachick et al., 2008). For the overall study, experiments were
performed at the NIAAA unless otherwise stated. In order to reduce the number of
mice used, but at the same time minimize potential carry-over effects due to,
e.g., stress of test exposure, some mice were tested on multiple assays (details
given below), with putatively more stressful tests later in a sequence and at
least 1 week between tests (unless otherwise stated). Mice were 2-10 months old
at the time of the experiments. On the basis of our previous finding that
schizophrenia-related phenotypes (Wiedholz et
al., 2008), as well fear-related and alcohol-related phenotypes
(Feyder et al., 2007; Palachick et al., 2008), in GluA1 KO did not vary as
a function of sex, the current study used both males and females in order to
increase the power of the analyses, without balancing sex ratio or considering
sex as a factor in the analyses. Another one of our studies found similar
behavioral results between male and female GluA1mice across a number of
measures (Bannerman et al., 2004).
TABLE 1
GluA1 are normal on simple measures of physical health, neurological and
sensory function
Physical health, sensory reflexes, motor, neurological functions and simple
behaviors in an empty cage were generally no different between genotypes. A
greater proportion of KO exhibited missing whiskers and bald patches,
forepaw clutching and defecation in an empty cage than WT. Unless a unit of
measurement is given in parenthesis, data are the percentage of mice within
each genotype showing a response (n=14/genotype). Redrawn from
(Wiedholz et al., 2008).
WT
KO
Physical health
Missing whiskers
20
47
Bald patches
13
27
Piloerection
0
0
Exophthalmus
0
0
Palpebral closure
0
0
Straub tail
0
0
Kinked tail
0
0
Kyphosis
0
0
Lordosis
0
0
Body weight (g)
21.5
22.9
Core body temp (°C)
36.5
36.3
Sensory reflexes
Approach response
100
100
Touch response
100
100
Palpebral response
100
80
Tail pink response
100
100
Hotplate paw withdrawal latency (sec)
11.49 ±0.86
9.67 ±0.94
Tail flick latency (sec)
2.02 ±0.07
1.85 ±0.15
Motor, neurological
Splayed limbs
0
0
Forepaw clutch
0
13
Hindpaw clutch
0
0
Empty cage behaviors
Wild running
0
0
Freezing
13
7
Trembling
0
0
Sniffing
100
100
Licking
0
0
Rearing
100
100
Jumping
0
0
Seizure
0
0
Defecation
20
60
Urination
7
13
Head bobbing
0
0
Circling
0
0
Abnormal gait
0
0
Retropulsion
0
7
Prancing forelimbs
0
0
NIAAA experiments
Mice were backcrossed to produce a >75% C57BL/6J
background, as verified by genome scan (Wiedholz et al., 2008). WT and KO were littermates bred from
heterozygous × heterozygous parents (to reduce potential influence
of maternal genotype (Millstein et al.,
2006)), either bred at The Jackson Laboratory and transported to
NIH at ∼8 weeks of age, or bred in-house. Non-mutant C57BL/6J mice
used in the GYKI 52466 experiments were males obtained from The Jackson
Laboratory and transported to NIH at ∼8 weeks of age. Mice were
housed in same-sex groupings in a temperature- and humidity-controlled
vivarium under a 12 h light/dark cycle (lights on 0600 h) and tested in the
light phase. Experimental procedures were performed in accordance with the
National Institutes of Health Guide for Care and Use of Laboratory Animals
and were approved by the local Animal Care and Use Committee. The number of
mice used in all experiments is given in the figure legends.
Oxford experiments
Mice were maintained on a C57BL/6J × CBA/J background. WT
and KO were littermates bred in-house from heterozygous ×
heterozygous parents. Mice were housed in same-sex groupings in a
temperature- and humidity-controlled vivarium under a 12 h light/dark cycle
(lights on 0700 h) and tested in the light phase. Experimental procedures
were approved by the Home Office.
Mannheim experiments
Mice were backcrossed to C57BL/6J for > 10 generations. WT
and KO were littermates bred in-house from heterozygous parents. Mice were
housed in a temperature- and humidity-controlled vivarium under a 12 h
reversed light/dark cycle (lights off 0600 h) and tested in the dark phase.
Experimental procedures were approved by the German animal welfare
authorities (Regierungspräsidium Karlsruhe).
Locomotor response to novelty and acute stress
As manic and psychotic episodes can be triggered by stress, we first
tested separate cohorts of mice for locomotor responses to 3 different
relatively mild stressors [1: a novel open field, 2: acute injection
stress (which is sufficient to activate the hypothalamic-pituitary-adrenal axis
in mice (Li et al., 2004)), and 3: acute
restraint stress], as well as activity in a non-stressful home cage-like
environment (Oxford).
Novel open field
The open field apparatus was a square arena (39 × 39
× 35 cm) with opaque white Plexiglas walls and floor. It was
evenly-illuminated to ∼60 lux. Mice (male WT=8, female
WT=7, male KO=8, female KO=7) were placed in a
corner and allowed to freely explore for 10 min. Total distance traveled and
time spent in the (20 × 20 cm) center was measured using the
Ethovision videotracking system (Noldus Information Technology, Leesburg,
VA). The effect of genotype was analyzed using Student's t-test.
Injection stress
Following a 30-min period of acclimation to the open field (as
above), mice (male WT=3, female WT=5, male KO=6,
female KO=1) were given an intraperitoneal (i.p.) injection of
0.9% saline (volume of 10 mL/kg body weight) and returned to the
open field. Total distance traveled was recorded for a further 30 min. For
all i.p. injections, mice were held in a level, supine position by the
experimenter, and injected in the abdomen. Injections were made midway
between the hip and midline, with the injection needle inserted at
∼30° angle.
Brief restraint stress
Following a 30-min period of acclimation to the open field (as
above), mice (male WT=7, female WT=3, male KO=4,
female KO=5) were removed and restrained in a 50 mL Falcon tube for
5 min before being returned to the open field for 30 min. For both stress
experiments, the effects of genotype and time on baseline pre-stress and
post-stress locomotor activity were analyzed using 2-factor analysis of
variance (ANOVA), with repeated measures for time, followed by
Bonferroni-Dunn post hoc tests. Stress-induced changes in
locomotor activity were analyzed by comparing the minute post-stress with
the minute pre-stress (i.e., minute 31 vs. 30).
Home cage-like assay (Oxford)
Mice (same as previously tested in the elevated plus-maze; male
WT=24, female WT=21, male KO=21, female
KO=26) were singly placed in a cage (22.5 × 12.5 ×
13 cm) with clean bedding and ad libitum food and water for
9.5 hr (09301900 h). Beginning at the onset of the dark phase (1900 h)
activity was measured primarily using the Med Associates Threshold system
(Med Associates Inc, St. Albans, VT). Threshold pressure pads convert
changes in pressure on pads into changes in voltage. The threshold range was
set to 20-50V, the time spent between these values being taken as time spent
moving. The effect of genotype was analyzed using Student's
t-test.
Response to novel and repeated forced swim stress
We next tested for behavioral responses to the more intense stress of
forced swimming. We examined responses to both acute and repeated (2 trials and
5 trials) forced swim test (FST) stress in separate cohorts of mice (apparatus
and procedure as described, Hefner and Holmes,
2007). To measure the HPA-axis response to acute swim stress, we
assayed blood corticosterone levels 30 min after a single FST (procedure as
described, Boyce-Rustay et al., 2007). To
analyze behavioral responses to repeated swim stress in greater detail, we
conducted a separate experiment (Oxford) using a modified version of the forced
swim test that distinguishes immobility, swimming and climbing behavior (Cryan et al., 2005).
2-trial forced swim
We first conducted a 2-trial procedure mimicking the original
procedure of Porsolt (Porsolt et al.,
1977) in which a 15-min trial 1 is followed by a shorter, 6-min,
trial 2 24 hr later. For each trial, mice (male WT=8, female
WT=7, male KO=8, female KO=7) were gently placed in
a 20 cm-diameter cylinder filled to ∼13 cm with 24
±1.0°C water (Hefner et al.,
2007) and scored for immobility (cessation of limb movements
except minor movement necessary to keep the mouse afloat) every 5 sec and
expressed as the percent number of instances of immobility during min 3-6 of
each trial. This design provides 1) a measure of immobility during min 3-6
of an initial exposure, equivalent to the standard forced swim test
procedure used for mice (Cryan and Holmes,
2005), and 2) a measure of the change in immobility produced by a
prior lengthy swim exposure. The effects of genotype and trial were analyzed
using 2-factor ANOVA, with repeated measures for trial, followed by
Bonferroni-Dunn post hoc tests.
5-trial forced swim
Here, we examined the development of immobility over an extensive
history of fixed-length, repeated swims (in a naïve cohort). Mice
(previously tested in the elevated plus-maze and home-cage activity tests;
male WT=7, female WT=11, male KO=10, female
KO=3) were given a 10-min trial each day for 5 consecutive days.
Immobility was scored during min 3-10 of each trial. The effects of genotype
and trial were analyzed using 2-factor ANOVA, with repeated measures for
trial, followed by Bonferroni-Dunn post hoc tests.
Corticosterone response to swim
A separate cohort of swim-naïve mice (male WT=3,
female WT=6, male KO=6, female KO=6) were exposed to
a single 10-min swim stress (as above) and returned to the home cage. Thirty
min later, mice were sacrificed (between 1000-1200 h) via rapid cervical
dislocation and decapitation to collect trunk blood. Non-stressed controls
were sacrificed at the same time. Blood samples were centrifuged at 13,000
rpm for 30 sec. Serum was extracted and assayed for total corticosterone
(bound and free) using the Coat-a-Count RIA TKRC1 kit (limit of detection:
5.7 ng/ml; Diagnostic Products Corp, Los Angeles) as previously described
(Boyce-Rustay et al., 2007). The
effects of genotype and stress were analyzed using 2-factor ANOVA.
Modified forced swim test (Oxford)
The apparatus and procedure were the same as for the 2-trial test
above with the exception that the cylinder was filled to 15 cm with water
and, in addition to immobility, swimming and climbing (movement while in
contact with the side of the cylinder in a near-vertical posture) were
analyzed during an identical window on both days between minutes 3-6 (male
WT=12, female WT=10, male KO=12, female
KO=14). The effects of genotype and trial were analyzed using
2-factor ANOVA, with repeated measures for trial, followed by
Bonferroni-Dunn post hoc tests.
Approach/avoidance behaviors in tests for anxiety-like behavior
We assessed GluA1 mutants in the elevated plus-maze - a test for
anxiety-like behavior based upon a conflict between avoidance and approach
(Cryan and Holmes, 2005). Because
abnormal mouse phenotypes in the elevated plus-maze appear prone to variation
across laboratories (Crabbe et al.,
1999), we conducted parallel elevated plus-maze experiments in the NIAAA
and Oxford laboratories. In addition, given evidence that different mouse
approach/avoidance tasks measure partly distinct forms of behavior (Brigman et al., 2009), we assessed the
GluA1 mutants in 2 other approach/avoidance tasks: the elevated zero-maze
(Mannheim) and light/dark emergence test (NIAAA). Finally, to further parse
anxiety- and novelty-seeking-related phenotypes, we tested for 1) stress-induced
hyperthermia, an anxiety assay (Groenink et al.,
1994), and 2) responses to repeated exposure to the elevated
plus-maze (Holmes et al., 2000).
Elevated plus-maze (NIAAA)
The apparatus consisted of 2 open arms (30 × 5 cm; 90 lux)
and 2 closed arms (30 × 5 × 15 cm; 20 lux) extending from a
5 × 5 cm central area and elevated 47 cm from the ground (San Diego
Instruments, San Diego, CA). The walls were made from black ABS plastic and
the floor from white ABS plastic. A 0.5 cm raised lip around the perimeter
of the open arms prevented mice from falling off the maze. Mice (previously
tested in the novel open field; male WT=7, female WT=7, male
KO=8, female KO=7) were placed in the center facing an open
arm and allowed to explore the apparatus for 5 min. Time spent in the open
arms, center square and closed arms, and entries into the open arms, center
square and closed arms was measured by the Ethovision videotracking system
(Noldus Information Technology Inc., Leesburg, VA), with the center of mass
of the mouse determining its arm location. The effect of genotype was
analyzed using Student's t-test.
Elevated plus-maze (Oxford)
The apparatus and procedure were the same as the NIAAA version with
the following exceptions: 1) the dimensions and lighting conditions were 35
× 6 cm (open arms, 85 lux), 35 × 6 × 20 cm (closed
arms, 10 lux) and 6 × 6 cm (center square) and elevated 70 cm from
the ground, and 2) the maze was made of dark gray plastic. Behavior was
measured by the Ethovision videotracking system, with 3 body points (front,
center and back of the body) determining its arm location. The effect of
genotype was analyzed using Student's t-test (same mice as tested in
the home cage-like assay).
Elevated zero-maze (Mannheim)
The apparatus consisted of an annular runway (width 6 cm, outer
diameter 46 cm, 50 cm above ground level) comprising 2 enclosed quadrants
(10 cm high inner and outer walls) separating 2 open quadrants (25 lux). The
walls and floor were made from gray plastic. Mice (all male) were placed in
a closed quadrant and allowed to explore the apparatus for 5 min, and
behavior was measured by the Ethovision videotracking system, with the
center of mass of the mouse determining its arm location. The effect of
genotype was analyzed using Student's t-test.
Light/dark emergence test
The apparatus comprised a square opaque black Plexiglas
‘shelter’ (16 × 16 × 19 cm) with a single
exit (6 × 4 cm) facing out into an open field arena (39 × 39
× 35 cm) with opaque white Plexiglas walls and floor that was
evenly-illuminated to ∼90 lux. Mice (previously tested in the novel
open field, and elevated plus-maze; male WT=8, female WT=7,
male KO=8, female KO=7) were placed in the shelter and
allowed to freely explore the whole apparatus for 5 min. Time out of the
shelter, number of shelter exits, and time and frequency of scans of the
open field from the shelter (head and <4 paws out of the shelter)
were manually measured using the Hindsight behavioral observation system
(Scientific Programming Services, Wokingham, UK). The effect of genotype was
analyzed using Student's t-test.
Stress-induced hyperthermia
Mice (previously assayed on the functional observation battery; male
WT=3, female WT=3, male KO=7, female KO=0)
were individually housed in a clean, empty cage for 5 hr to avoid
disturbance resulting from handling of cage mates (Van der Heyden et al., 1997). Core body
temperature was measured using a peanut oil-lubricated physiological
thermometer probe (Thermalert TH-5, Physitemp, Clifton, NJ) inserted 2 cm
into the rectum for ∼10 sec on 2 occasions separated by 10 min.
Stress-induced hyperthermia is the increase in core body temperature between
the 2 measurements. The effect of genotype was analyzed using
Student's t-test.
Repeated exposure to elevated plus-maze
Test-naïve mice (male WT=13, female WT=9,
male KO=9, female KO=9) were tested as above (NIAAA version)
over 2 trials, separated by 24 hr. The effects of genotype and trial were
analyzed using 2-factor ANOVA, with repeated measures for trial, followed by
Bonferroni-Dunn post hoc tests.
Effects of AMPAR/kainate antagonist GYKI 52466
Behavioral abnormalities in GluA1 KO could arise from either loss of
GluA1 function in the adult brain or indirect abnormalities arising from
alterations in neural development. One indirect way to address this issue is to
ask whether pharmacological inactivation of GluA1 in adult non-mutant mice
phenocopies the effects of constitutive GluA1 KO. There are currently no
GluA1-selective antagonists, precluding a direct comparison. However, the
antagonist GYKI 52466 has relative selectivity for AMPA and kainate receptors
over other glutamate receptors and has behavioral effects in rats and NSA mice
(Tzschentke and Schmidt, 1997; Vanover, 1998). We tested the effects of
systemic GYKI 52466 in non-mutant C57BL/6J mice (genetic background of GluA1 KO;
all male) on novel open field and elevated plus-maze assays (in the same mice)
under the same conditions which produce a robust phenotype in GluA1 KO.The novel open field and elevated plus-maze tests used to test C57BL/6J
mice involved the same apparatuses and procedures as described above (NIAAA
version). For each experiment, mice were tested 30 min after treatment with 0,
0.5, 2.5, 5, or 10 mg/kg GYKI 52466 (Sigma, St. Louis, MO, dissolved in a
vehicle of 10% Dimethyl sulfoxide (DMSO) and 90% 0.9%
saline) injected i.p. in a volume of 10 mL/kg body weight. This vehicle did not
produce any observable behavioral effects. Doses were chosen on the basis of
previous behavioral studies in mice (Kapus et
al., 2008; Vekovischeva et al.,
2007). The effect of dose was analyzed using ANOVA.GluA1 KO have redistribution of GluA2/3 (Zamanillo et al., 1999), and it remains possible that there is a
compensatory functional upregulation of AMPAR. Therefore, we tested whether the
effects of GYKI 52466 in the novel open field were altered in KO, as a probe for
effects on GluA2/3 in the mutants (male WT=3, female WT=8, male
KO=6, female KO=0). Test-naïve mice were injected i.p.
with 0 or 10 mg/kg GYKI 52466 and immediately tested in a novel open field for
30 min. A within-subjects Latin square design was employed, in which half the
mice received vehicle one day and drug the next day, and vice versa for the
other half. The effect of genotype and treatment was analyzed using ANOVA, with
repeated measures for treatment.
Responses to psychostimulants
Prior studies have consistently demonstrated novelty-induced locomotor
hyperactivity in GluA1 KO (Bannerman et al.,
2004; Chourbaji et al., 2008;
Vekovischeva et al., 2004; Wiedholz et al., 2008). This phenotype is
potentially relevant to a number of neuropsychiatric conditions (e.g.,
schizophrenia, bipolar disorder, ADHD), but does not discriminate between them.
By contrast, psychostimulants such as amphetamine (Adderall) and methylphenidate
(Ritalin) would be predicted to exacerbate a bipolar- or schizophrenia-related
phenotype (Anand et al., 2000; Einat and Manji, 2006), but normalize an
ADHD-related phenotype given their therapeutic efficacy for ADHD. We therefore
tested test-naïve separate cohorts of GluA1 KO for locomotor responses
to hyperlocomotor-inducing (sub-stereotypic) doses of amphetamine and
methylphenidate.We tested the hyperlocomotor-inducing effects of amphetamine using a
within-subjects experimental design previously used to test for mania-related
phenotypes in GluA6 KO mice (Shaltiel et al.,
2008). Mice (male and female counts not determined) were given a 60
min period of habituation to the open field and then injected with 2 mg/kg
amphetamine (Sigma, St. Louis, MO, dissolved in 0.9% saline and injected
i.p. in a volume of 10 mL/kg body weight) and returned to the open field for 10
min. The effect of genotype and (10-min) pre- vs. (10-min) post-drug period was
analyzed using ANOVA, with repeated measures for period, followed by
Bonferroni-Dunn post hoc tests and Bonferroni-corrected
t-tests. In addition, the effect of genotype on the drug-induced increase in
total distance traveled (=post-drug minus pre-drug) was analyzed using
Student's t-test.We tested the hyperlocomotor-inducing effects of methylphenidate in a
separate cohort, using a between-subjects design. Mice (male WT=8,
female WT=10, male KO=12, female KO=6) were given a 60
min period of habituation to the open field and then injected with vehicle or 5
mg/kg methylphenidate (Sigma, St. Louis, MO, dissolved in 0.9% saline
and injected i.p. in a volume of 10 mL/kg body weight) and returned to the open
field for 10 min. Methylphenidate-induced locomotor activity was measured as the
difference in drug relative to vehicle locomotor activity. The effect of
genotype and drug was analyzed using ANOVA. In addition, the effect of genotype
on the drug-induced increase in total distance traveled (=drug minus
vehicle) was analyzed using Student's t-test.
Effects of rapid dopamine depletion
Impaired dopaminergic function is implicated in schizophrenia and
bipolar disorder. We previously found that GluA1 KO have impaired dopamine
clearance in the striatum, and that the KO hyperlocomotor phenotype was rescued
by treatment with the dopamine D2 receptor antagonist haloperidol (Wiedholz et al., 2008). These data suggest
that excessive striatal dopamine may underlie the GluA1 KO hyperlocomotor
phenotype. To test this hypothesis, we examined the effects of rapid depletion
of dopamine (via treatment with the tyrosine hydroxylase inhibitor
α-methyl-p-tyrosine methyl ester (AMPT)) on locomotor activity (Costa et al., 2006; Gainetdinov et al., 1999). To verify depletion,
striatal dopamine (and serotonin) tissue content, as well as metabolites of
these two neurotransmitters, was measured immediately after testing.Mice (previously tested in stress-induced hyperthermia assay; male
WT=16, female WT=15, male KO=14, female KO=10)
were injected i.p. (volume of 10 mL/kg body weight) with 0 or 200 mg/kg AMPT
(Sigma, St. Louis, MO, dissolved in 0.9% saline) and, 60 min later,
tested in a novel open field (apparatus and procedure as described above) for 30
min. Dose was selected based on pilot work and previous studies (Costa et al., 2006; Gainetdinov et al., 1999) to cause significant dopamine depletion
but not significant locomotor hypoactivity in WT. The effect of genotype and
treatment was analyzed using ANOVA, followed by Bonferroni-Dunn post
hoc tests.Immediately after open field testing, a subset of mice (male
WT=11, female WT=10, male KO=14, female KO=6)
were sacrificed via cervical dislocation and decapitation to verify reduced
striatal dopamine content via high performance liquid chromatography (HPLC), as
previously described (Boyce-Rustay et al.,
2008). A dissection of the striatum (also containing septum) was made
on ice and tissue was frozen at -80°C. Frozen samples were homogenized
by ultrasonic processing in 800 μL of 0.1 M perchloric acid containing
1% ethanol and 0.02% EDTA and centrifuged for 20 min at 3000 g.
Thirty μL of the homogenate was used for analysis using a Luna
5μC18(2), 250 × 2.0 mm column (Phenomenex 00G-4252-B0, Torrance,
CA) held at 30°C, Waters Corporation (Milford, MA) 717plus autosampler
at 4°C, 510 pump at 0.4 ml/min and amperometric electrochemical detector
(EiCOM CB100) set at Eox. 0.82 V. The mobile phase contained 2.8 g
1-heptanesulfonic acid sodium salt, 0.17 g EDTA, 20 ml triethylamine, dissolved
in 2.2 L water, pH adjusted to 2.5 with 13 ml 85% phosphoric acid, plus
90 ml acetonitrile. Adjusted to 1 L total volume, these values are: 1.21 g
1-heptanesulfonic acid sodium salt, 0.073 g EDTA, 8.61 ml triethylamine,
dissolved in 947.1 ml water, pH adjusted to 2.5 with 5.60 ml 85%
phosphoric acid, plus 38.74 ml acetonitrile. The detector output was recorded
and analyzed with Waters Empower 2 Chromatography Data Software. No internal
standard was used for this assay. The quantification was against external
standards injected several times during the run (before the samples, every 12
samples, and post-sample injections). We examined tissue content levels of
dopamine and its monoamine metabolites 3,4-dihydroxyphenylacetic acid (DOPAC),
homovanillic acid (HVA), and its catechol-O-methyltransferase
metabolite 3-methoxytyramine (3-MT), as well as norepinephrine (NE), and
5-hydroxytryptamine (5-HT) and its monoamine metabolite 5-hydroxyindole-3-acetic
acid (5-HIAA). The effect of genotype and treatment was analyzed using ANOVA,
followed by Bonferroni-Dunn post hoc tests.
Effects of GSK-3β inhibitor
There is growing evidence supporting the contribution of glycogen
synthase kinase-3 beta (GSK-3β) to the pathophysiology and treatment of
schizophrenia and bipolar disorder (Gould and
Manji, 2002). We therefore asked whether GSK-3β inhibition
would normalize the locomotor hyperactivity and forced swim abnormalities in
GluA1 KO by treating mice with 2 mg/kg SB216763 every other day for 11 days
(i.e., 6 treatments in total, similar to Mao et
al., 2009) and subsequently testing in the open field and repeated
FST assays. To mimic the procedure used by Mao et al., we tested mice in both
the open field and repeated FST assays.Test-naïve mice (male WT=12, female WT=14, male
KO=11, female KO=15) were treated with 2 mg/kg SB216763 (Sigma,
St. Louis, MO, dissolved in 90% 0.9% saline/10% DMSO and
injected i.p. in a volume of 10 mL/kg body weight) every other day for 10 days
(i.e., as previously described (Mao et al.,
2009)). On day 10, mice were tested in the open field for 10 min
(apparatus and procedure as described above). Mice received another drug
treatment on day 11, and on days 12 and 13 were given a 15 min and then 6-min
forced swim exposure, respectively (apparatus and procedure as described above).
The effect of genotype and treatment was analyzed using ANOVA.
Effects of lithium treatment
A key test of whether GluA1 KO behavioral abnormalities are
mania-related is whether they are rescued by treatment with an anti-manic drug
such as lithium (O'Donnell and Gould,
2007). We chronically treated test-naïve mice with lithium
for 14 days (Gould et al., 2007; Shaltiel et al., 2008) and then over
subsequent days (while still on-drug) tested in the novel open field (male
WT=13, female WT=18, male KO=9, female KO=20)
and elevated plus-maze (male WT=6, female WT=12, male
KO=6, female KO=10). Because the PKC pathway has been implicated
in bipolar disorder and as a target for lithium (Szabo et al., 2009), we probed this pathway at baseline and after
lithium treatment by quantifying phosphorylation of the PKC activity markers
myristoylated alanine-rich C kinase (MARCKS; male WT=5, female
WT=6, male KO=6, female KO=6) and neuromodulin (growth
associated protein 43, GAP43; male WT=5, female WT=7, male
KO=6, female KO=6). (Note, to avoid potentially confounding
effects of stress on these molecular measures, we did not test for lithium
effects on forced swim test behavior in this experiment).Regular rodent chow was loaded with 4 g/kg lithium carbonate (Bio-Serv,
Frenchtown, NJ, USA) to produce brain lithium levels of ∼0.55 mM and
plasma levels in the human therapeutic range (∼1.0 mM) (Shaltiel et al., 2008). Non-treated controls received
the same chow with no lithium. Because lithium produces polyuria and polydipsia,
all mice (including controls) had their chow moistened daily in 0.9%
saline, and cage bedding was changed approximately three times weekly. On day
15, mice were tested in the open field for 10 min (apparatus and procedure as
described above), and the data analyzed in 2-min timebins to investigate
within-session effects of lithium. On day 16, mice were tested in the elevated
plus-maze (NIAAA; apparatus and procedure as described above). The effect of
genotype and treatment was analyzed using ANOVA, followed by Bonferroni-Dunn
post hoc tests.On day 17, mice were sacrificed by cervical dislocation and rapid
decapitation. With reference to a mouse atlas (Paxinos and Franklin, 2001), the ventral striatum (∼
+1.00 - +0.80 mm AP from Bregma) and ventromedial prefrontal
cortex (∼ +1.90 - +1.70 mm AP from Bregma) were
dissected by micropunch on ice, flash frozen in liquid nitrogen and stored at
-80°C until analysis. Samples were sonicated in Homogenization Buffer A
(50 mM Tris-Cl, pH 7.5, containing 2 mM dithiothreitol, 2 mM EDTA, 2 mM EGTA, 50
μM 4-(2-aminoethyl)-benzenesulfonylfluoride hydrochloride, 50 mM KF, 50
nM okadaic acid, 1 mM sodium orthovanidate, 5 mM sodium pyrophosphate,
0.1% NP-40, and 5 μg/ml each of leupeptin, aprotinin,
chymostatin, and pepstatin A), spun in the Eppendorf 5810R centrifuge (Westbury,
NY) for 20 minutes at 4°C at 20,000 rcf, and the clear homogenate was
used as total protein. Aliquots of crude whole-cell homogenates taken from the
frontal cortices of mice were used to determine the content of phosphorylated
and total protein. Protein concentrations were determined using the Bio-Rad
(Hercules, CA) protein assay kit, and the linearity of the protein concentration
for immunoblotting was ascertained by resolution of selected concentrations of
protein. Equal amounts of proteins were subjected to 10% SDS-PAGE gels
and separated by electrophoresis. β-actin was used as an internal
control, with no differences observed between genotypes. Proteins were then
electrophoretically transferred to nitrocellulose membranes. Nonspecific binding
on the nitrocellulose was blocked with Tris
Buffered Saline plus
Tween 20 (TBST), 10% nonfat dry milk, and
then incubated with anti-phospho-GAP43 antibody (Upstate Laboratories, Syracuse,
NY), anti-GAP43 antibody (Upstate Laboratories, Syracuse, NY), anti-MARCKS
antibody (Calbiochem, Gibbstown, NJ), and anti-Phospho-MARCKS (Ser 152/156)
antibody (Cell Signaling Technology, Danvers, MA). The secondary antibodies were
horseradish peroxidase-conjugated goat anti-rabbit IgG and goat anti-mouse IgG
(Cell Signaling Technology, Danvers, MA). The ECL plus kit (GE Healthcare,
Piscataway, NJ) was used as a detection system. Notably, in these experiments,
nitrocellulose membranes were first probed with anti-phospho-MARCKS,
anti-phospho-GAP43 and then stripped with stripping buffer and re-probed with
the anti-MARCKSand anti-GAP43 antibodies. Quantification of the immunoblots was
performed by densitometric scanning of the x-ray film using a Kodak Image
Station 440 CF and Kodak 1D Image Analysis Software (Eastman Kodak, Rochester,
NY). For each gel, the net and sum intensity was determined by the software. Net
intensity within each gel was normalized to the averaged gel-value from
control-treated WT and the effect of genotype analyzed using Student's
t-test.
Results
GluA1 KO exhibited locomotor hyperactivity in response to novelty and mild
stress
KO traveled significantly farther than WT in a novel open field
(t=9.16, df=27, p<.01) (Figure 1A). By contrast, movement in a home cage-like
environment was no different between genotypes (Figure 1B). KO traveled significantly farther than WT before
injection stress (main effect of genotype: F1,13=123.92,
p<.01). Injection stress produced a transient (min
31 vs. min 30) decrease in locomotor activity in WT but an increase in activity
in KO (genotype × time interaction: F28,364=6.03,
p<.01) (Figure
1C). A separate cohort of KO traveled significantly farther than WT
before restraint stress (main effect of genotype: F1,16=31.37,
p<.01). Restraint stress produced a transient (min
31 vs. min 30) increase in locomotor activity in both genotypes, but a greater
increase in KO (genotype × time interaction: F29,464=3.41,
p<.01) (Figure
1D).
FIGURE 1
GluA1 KO exhibited locomotor hyperactivity in response to novelty and
mild stress
(A) KO traveled significantly farther than WT in a 10 min exposure to a novel
open field (**p<.01)
(n=15/genotype). (B) Movement in a home cage-like environment was
not different between genotypes (n=45-47/genotype). (C) KO traveled
significantly farther than WT before injection stress. Injection stress
produced a transient decrease in locomotor activity in WT but an increase in
activity in KO (*p<.05 vs. minute 31 in WT;
#p<.05 vs. minute 30 in same genotype)
(n=7-8/genotype). (D) KO traveled significantly farther than WT
before restraint stress. Restraint stress produced a transient increase in
locomotor activity in both genotypes, but a greater increase in KO
(n=9-10/genotype). Data are Means ±SEM.
GluA1 KO showed decreased immobility during forced swim
KO exhibited significantly less immobility than WT over each of 2 FST
trials, although the magnitude of the difference was greater on trial 1 than
trial 2 (genotype × trial interaction: F1,28=21.34,
P<.01) and both genotypes showed a significant increase in immobility
across trials (Figure 2A). When a separate
cohort was tested over 5 × 10-min FST trials, KO displayed significantly
less immobility than WT during trial 1 but not trials 2-5 (genotype ×
trial interaction: F4,116=7.49, p<.01) (Figure 2B). Post hoc tests
revealed that KO, but not WT, showed a significant increase in immobility by
trial 3, as compared to trial 1. In a swim-naïve cohort, serum
corticosterone was similarly elevated in WT and KO after a single FST trial,
relative to non-stressed baseline (main effect of stress: F1,17=12.51,
p<.01; main effect of genotype:
ns; stress × genotype interaction: ns)
(Figure 2C).
FIGURE 2
GluA1 KO showed decreased immobility in the forced swim test
(A) KO exhibited significantly less immobility than WT over each of 2 FST
trials, although the effect was larger during min 3-6 of a 15-min trial 1
than min 3-6 of a 6-min trial 2
(**p<.01, vs. WT/same trial). WT
and KO both showed increased immobility from trial 1 to 2
(##p<.01 vs. trial 1/same
genotype) (n=15/genotype). (B) When tested over 5 × 10 min
FST trials, KO displayed less immobility than WT during trial 1
(*p<.05) but not trials 2-5. KO showed
a significant increase in immobility by trial 3
(#p<.05) (n=13-18/genotype). (C)
Serum corticosterone was similarly elevated in WT and KO after a single FST
trial, relative to non-stressed baseline
(†p<.05 vs. base)
(n=4-6/genotype/stress). Data are Means ±SEM.
GluA1 KO showed increased swimming in a modified forced swim test
KO showed significantly less immobility (genotype × trial
interaction: F1,46=18.98, p<.01) and more
swimming (genotype × trial interaction: F1,46=21.54,
p<.01), but no difference in climbing (all effects:
ns), relative to WT, on trial 1 (Figure 3A,B) but not trial 2 (Figure 3C,D). KO, but not WT, showed a significant
increase in immobility and a decrease in swimming from trial 1 to 2.
FIGURE 3
GluA1 KO showed increased swimming in a modified forced swim test
(A) KO showed significantly less immobility and more swimming on trial 1
(**p<.01 vs. WT). (B) Climbing
did not differ between genotypes on trial 1. (C) KO showed an increase in
immobility and a decrease in swimming on trial 2, relative to trial 1, and
did not differ from WT in either behavior on this trial
(##p<.01 vs. trial 1/KO). (D)
Climbing did not differ between genotypes on trial 2.
n=22-26/genotype. Data are Means ±SEM.
GluA1 KO showed increased open arm/quadrant exploration in elevated maze
tests
In the elevated plus-maze (NIAAA), KO made significantly more open
(t=3.10, df=25, p<.01) and center
(t=2.53, df=25, p<.05) but not closed
entries than WT (Figure 4A). KO also had
significantly more center (t=3.62, df=25,
p<.01) time and a trend for more open time
(t=1.97, df=25, p=.0605), but less
closed time (t=6.56, df=25, p<.01) than
WT (Figure 4B).
FIGURE 4
GluA1 KO showed increased open arm/quadrant entries and increased center
time in elevated maze tests
(A) In the NIAAA elevated plus-maze, KO made more open and center, but not
closed, entries than WT (*p<.05 vs. WT)
(n=14-15/genotype). (B) KO showed more center time and less closed
time, and a trend for more open time, as compared to WT
(**p<.01 vs. WT). (C) In the
Oxford elevated plus-maze, KO made more open and center, but not closed,
entries than WT (**p<.01 vs. WT)
(n=45-47/genotype). (D) KO showed more center time and less closed
time, and a trend for more open time, as compared to WT
(**p<.01 vs. WT). (E) In the
elevated zero-maze (Mannheim), KO made fewer open entries
(**p<.01) and (F) showed a
non-significant trend for less open quadrant time than WT
(n=7-8/genotype). Data are Means ±SEM.
In the elevated plus-maze (Oxford), KO made significantly more open
(t=3.41, df=90, p<.01) and center
(t=4.63, df=90, p<.01) but not closed
entries than WT (Figure 4C). KO also had
significantly more center (t=2.78, df=90,
p<.01) time and a trend for more open time
(t=1.90, df=90, p=.0608), but less
closed time (t=10.06, df=90, p<.01)
than WT (Figure 4D).In the elevated zero-maze (Mannheim), KO made significantly fewer open
entries (t=3.36, df=13, p<.01) (Figure 4E) and showed a non-significant trend
for less open quadrant time (t=2.10, df=13,
p=.0554) than WT (Figure
4F).
GluA1 KO showed increased risk assessment and stress-induced
hyperthermia
In the light/dark emergence test, KO made significantly more shelter
exits (t=2.15, df=26, p<.05) and showed
more frequent scanning from the shelter (t=2.20, df=26,
p<.05) than WT (Figure 5A). KO did not spend significantly more time out of the
shelter than WT, but engaged in more time scanning than WT (t=2.34,
df=26, p<.05) (Figure 5B).
FIGURE 5
GluA1 KO showed increased exits and risk assessment in the light/dark
emergence test and a trend for greater stress-induced hyperthermia
(A) In the light/dark emergence test, KO made more shelter exits and showed
more frequent scanning than WT (*p<.05 vs.
WT) (n=15/genotype). (B) KO did not spend significantly more time
out of the shelter than WT, but engaged in more time scanning from the
shelter than WT (*p<.05 vs. WT). (C) KO
showed a trend for greater stress-induced hyperthermia than WT
(n=6-7/genotype). (D) In the elevated plus-maze, KO made
significantly more open entries than WT, regardless of trial
(n=18-22/genotype). Data are Means ±SEM.
KO showed a near significant trend for greater stress-induced
hyperthermia than WT (t=2.12, df=11,
p=.0580) (Figure
5C). Basal temperature was significantly higher in WT than KO
(WT=36.7 ±.42, KO=35.7 ±.19; t=2.32,
df=11, p<.05).In a naïve cohort tested over 2 exposures to the elevated
plus-maze (NIAAA), KO made significantly more open entries than WT, regardless
of trial (main effect of genotype: F1,38=24.79,
p<.01, main effect of trial: ns,
genotype × trial interaction: ns) (Figure 5D). KO also showed significantly more open
time than WT regardless of trial (main effect of genotype: F1,38=11.24,
p<.01; main effect of trial: ns;
genotype × trial interaction: ns) (WT/trial 1
(sec)=15.0±2.4, KO/trial 1=26.1±3.7, WT/trial
2=12.2±3.1, KO/trial 2=30.0±4.7). Closed arm
entries were not different between genotypes on trial 1, but were greater in KO
than WT on trial 2 (genotype × trial interaction: F1,38=4.94,
p<.05; WT/trial 1=15.3±1.2,
KO/trial 1=15.4±1.5, WT/trial 2=14.3±1.5,
KO/trial 2=20.0±2.3).
GYKI 52466 did not mimic GluA1 locomotor phenotype in C57BL/6J, or alter
GluA1 KO phenotype
GYKI 52466 treatment did not significantly alter open field locomotor
activity or elevated plus-maze behavior, relative to vehicle, in non-mutant
C57BL/6J mice (Table 2). Note, although
GYKI 52466 and other AMPAR antagonists exhibit anxiolytic-like effects in rats
(Alt et al., 2006; da Cunha et al., 2008; Kapus et al., 2008; Kotlinska and Liljequist, 1998; Matheus and Guimaraes, 1997; Turski
et al., 1992), previous work in NMRI mice (light/dark emergence test)
(Kapus et al., 2008) and Turku
Aggressive mice (social interaction test) (Vekovischeva et al., 2007) found negative (as here) or
anxiogenic-like effects.
TABLE 2
Effects of AMPA/kainate antagonist GYKI 52466 in non-mutant C57BL/6J and
GluA1 KO
GYKI 52466 did not affect novel open field locomotor activity or elevated
plus-maze anxiety-related behavior (n=8-9/dose) in C57BL/6J. GYKI
52466 did not alter the GluA1 KO open field locomotor hyperactivity
phenotype (n=6-11/genotype). Data are means ±SEM.
C57BL/6J
GYKI 52466 dose (mg/kg)
0
0.5
2.5
5
10
Novel open field
locomotor activity
Total distance traveled (m)
41.9 ±2.0
44.5 ±3.7
49.0 ±2.3
47.6 ±3.3
40.3 ±2.6
Elevated plus-maze
anxiety-related behavior
Open arm entries
5.6 ±1.0
5.1 ±1.4
6.1 ±1.1
6.4 ±0.7
7.6 ±1.4
Closed arm entries
22.3 ±1.5
21.4 ±1.6
19.9 ±1.5
20.3 ±1.3
24.6 ±1.5
%Time in open arms
7.4 ±1.8
6.4 ±2.4
9.7 ±2.7
9.8 ±2.2
13.6 ±3.5
%Time in closed arms
58.2 ±1.6
56.3 ±1.8
59.5 ±3.1
59.2 ±2.7
61.6 ±2.9
GluA1 KO
Locomotor
hyperactivity
WT/VEH
WT/GYKI
KO/VEH
KO/GYKI
Total distance traveled (m)
87.7 ±6.8
81.6 ±8.6
168.5 ±12.3
157.2 ±18.2
In KO, GYKI 52466 treatment did not alter the open field locomotor
hyperactivity phenotype (main effect of genotype: F1,15=35.33,
p<.01; main effect of drug: ns;
genotype × drug interaction: ns) (Table 2).
Psychostimulants exacerbated GluA1 KO locomotor phenotype
Treatment with amphetamine increased total distance traveled relative to
pre-drug baseline in both WT and KO (drug × genotype interaction:
F1,17=5.27, p<.05; WT drug vs. baseline
Bonferroni correct t-test: t=3.24, df=9,
p<.05; KO drug vs. baseline Bonferroni correct t-test:
t=4.17, df=8, p<.01) (Figure 6A). However, there was a significantly greater
drug-induced increase (relative to pre-drug baseline) in KO than WT
(t=2.32, df=16, p<.05) (Figure 6A, inset). Total distance traveled was greater
in KO than WT after amphetamine treatment, but not during pre-drug baseline
activity (probably because this baseline comprised the last 10 min of a 60-min
acclimation period, with no injection).
(A) Amphetamine produced a significant increase in open field total distance
traveled in both genotypes (#p<.05,
##p<.01 vs. baseline). KO given
amphetamine traveled significantly farther than WT given this drug
(**p<.01). There was a significantly greater
drug-induced increase in locomotor activity in KO than WT (inset)
(*p<.05) (n=9/genotype). (B)
Methylphenidate significantly increased total distance traveled in both
genotypes. The drug-induced increase was significantly greater in KO than WT
(inset) (*p<.05)
(n=9/genotype/treatment). Data are Means ±SEM.
In a separate cohort, treatment with methylphenidate increased total
distance traveled relative to vehicle in both WT and KO, and KO traveled farther
than WT regardless of treatment (main effect of genotype: F1,32=157.57,
p<.01; main effect of drug: F1,32=30.96,
p<.01; genotype × drug interaction:
ns). However, despite the absence of a genotype ×
drug interaction, methylphenidate produced a significantly greater increase in
locomotor activity in KO than WT when measured as the increase from vehicle
(t=2.30, df=17, p<.05) (Figure 6B, inset).
Rapid dopamine depletion paradoxically exacerbated GluA1 KO locomotor
phenotype
Vehicle treated KO traveled significantly farther than WT, and AMPT
treatment produced an additional significant increase in KO, but had no effect
in WT (genotype × treatment interaction: F2,51=7.90,
p<.01) (Table
3). Post mortem striatal tissue levels of monoamines
and their metabolites did not differ between genotypes at baseline (all main
effects of genotype: ns). AMPT treatment significantly
decreased striatal dopamine (main effect of treatment: F1,37=24.49,
p<.01), DOPAC (main effect of treatment:
F1,37=81.37, p<.01), HVA (main effect of
treatment: F1,37=44.31, p<.01), and 3-MT (main
effect of treatment: F1,37=20.50, p<.01), irrespective of
genotype (Table 3). Norepinephrine
content was unaffected by treatment or genotype. AMPT treatment significantly
increased striatal tissue levels of 5-HT regardless of genotype (main effect of
treatment: F1,37=9.27, p<.01), but increased
5-HIAA only in KO (genotype × treatment interaction: F1,37=7.29,
p<.05) (Table
3).
TABLE 3
Rapid dopamine depletion by AMPT paradoxically exacerbated GluA1
locomotor hyperactivity
Vehicle treated KO traveled significantly farther than WT, whereas AMPT
treatment produced a further increase in KO but had no effect in WT
(&&p<.01 vs. WT/same treatment;
#p<.05 vs. KO/vehicle)
(n=12-16/genotype/treatment). AMPT treatment decreased striatal
tissue levels (ng/g tissue) of dopamine, DOPAC, HVA, and 3-MT, irrespective
of genotype (n=10-11/genotype/treatment)
(**p<0.01). AMPT treatment significantly increased
striatal serotonin regardless of genotype
(††p<0.01), but increased 5-HIAA only in KO
(#p<.05 vs. KO/vehicle). Norepinephrine
content was unaffected by treatment or genotype. Data are Means
±SEM.
WT
KO
VEH
AMPT
VEH
AMPT
Novel open field
Total distance traveled (m)
61.6 ±5.9
49.2 ±4.2
115.2
±11.7&&
155.9±15.4&&#
Striatal monoamine
levels
Dopamine**
3555.8 ±599.1
937.5 ±281.9
2797.6 ±461.5
1235.1 ±285.8
DOPAC**
344.7 ±32.9
80.8 ±15.3
270.8 ±33.9
84.8 ±10.1
HVA**
649.6 ±76.6
196.2 ±26.4
561.4 ±79.4
241.3 ±34.3
3-MT**
123.8 ±17.1
31.9 ±10.7
93.2 ±18.1
50.2 ±13.2
Serotonin††
1080.6 ±46.9
1202.3 ±65.3
1054.7 ±64.9
1343.2 ±86.4
5-HIAA
657.8 ±49.2
557.7 ±48.3
540.8 ±41.5
720.8 ±65.9#
Norepinephrine
565.6 ±55.0
569.5 ±55.2
685.4 ±58.6
578.9 ±48.6
GSK-3β inhibitor did not rescue GluA1 KO locomotor phenotype
KO traveled significantly farther than WT, regardless of treatment,
although there was a borderline genotype × treatment interaction (main
effect of genotype: F1,47=33.37, p<.01; main
effect of treatment: ns; genotype × treatment
interaction: F1,47=3.55, p=.0657) due to a
trend for SB216763 treatment to reduce locomotor hyperactivity in KO (Table 4). KO showed significantly less
immobility than WT across 2 FST trials, regardless of SB216763 treatment (main
effect of genotype: F1,48=21.65, p<.01: main
effect and interactions with treatment: ns) (Table 4). Immobility increased from trial 1 to 2
regardless of genotype or treatment (main effect of trial: F1,48=27.58,
p<.01).
TABLE 4
GSK-3β inhibitor did not rescue GluA1 locomotor phenotype
KO traveled significantly farther than WT, regardless of treatment, although
there was a trend for SB216763 treatment to reduce locomotor hyperactivity
in KO (n=13/genotype/treatment). KO showed significantly less
immobility than WT across 2 FST trials, regardless of SB216763 treatment.
Immobility (min 3-6) increased from trial 1 to 2 regardless of genotype or
treatment. (n=13/genotype/treatment; same mice as for novel open
field test). Data are Means ±SEM.
WT
KO
VEH
SB216763
VEH
SB216763
Novel open field
Total distance traveled (m)
36.4 ±4.7
34.8 ±6.1
71.7 ±9.1
55.6 ±3.4
Forced swim test
Trial 1 percent immobility
34.1 ±7.0
39.4 ±6.4
12.7 ±3.0
12.5 ±3.5
Trial 2 percent immobility
49.7 ±7.5
62.7 ±6.9
30.6 ±7.6
35.1 ±7.2
Lithium partially rescued GluA1 KO phenotype
In the elevated plus-maze, KO receiving control treatment, but not
lithium treatment, made significantly more open entries than WT (genotype
× treatment interaction: F1,30=5.12,
p<.05) (Figure 7A)
and showed a near significant trend for more percent open time than WT
(WT/control=17.0 ±3.0, WT/lithium=14.8 ±3.7,
KO/control=48.3 ±5.5, KO/lithium=22.0 ±11.1;
genotype × treatment interaction: F1,30=4.06,
p=.053). Two lithium-treated KO that made no arm
entries were excluded from the plus-maze analysis. Closed arm entries was
unaffected by genotype or treatment (data not shown).
FIGURE 7
Lithium partially rescued GluA1 locomotor and PKC phenotype
(A) In the elevated plus-maze, KO receiving control treatment, but not
lithium treatment, made significantly more open entries than WT
(n=7-9/genotype/treatment)
(**p<.01 vs. WT/control;
#p<.05 vs. KO/control). (B) In the
novel open field, control KO were more active than control WT for all 2-min
timebins, and lithium treatment reduced activity during the first timebin in
both genotypes such that activity in lithium treated KO was normalized to WT
control levels. Lithium treatment also reduced activity in KO, relative to
control treated KO, during the second timebin but was ineffective in
timebins thereafter. In the fourth and fifth timebins, lithium treatment
increased activity in WT. (*p<.01
KO/control vs. WT/control, #p<.05 lithium
vs. control/same genotype) (n=14-17/genotype/treatment). (C) Levels
of phospho-MARCKS in PFC were significantly higher in control-treated but
not lithium-treated KO relative to WT (n=5-6/genotype/treatment).
(D) Levels of phospho-neuromodulin in PFC were also significantly higher in
control-treated but not lithium-treated KO relative to WT
(n=6/genotype/treatment).
(**p<.01 vs. WT/control;
##p<.01,
#p<.05 vs. KO/control). Data are Means
±SEM.
In the novel open field (Figure
7B), there was a significant main effect of genotype
(F1,56=151.83, p<.01), as well as a significant
interaction between genotype and 2-min timebin (F4,224=18.72,
p<.01) and treatment and timebin
(F4,224=11.07, p<.01) for total distance
traveled. Post hoc tests showed that whereas control diet KO were more active
than control diet WT for all timebins, lithium treatment reduced activity during
the first 2-min timebin in both genotypes such that activity in lithium treated
KO was normalized to WT control levels. Lithium treatment also reduced activity
in KO, relative to control treated KO, during the second 2-min timebin but was
ineffective in timebins thereafter. In the fourth and fifth timebins, lithium
treatment increased activity in WT. One lithium-treated WT had a seizure at the
start of the test, and was excluded from open field analysis. Three other mice
(1 control chow-treated KO, 2 lithium-treated WT) were greater or less than 2
standard deviation outliers for total distance traveled for their treatment
group, and were excluded from this analysis. Plasma lithium levels measured
after the open field were in the therapeutic range in WT (1.05 ±0.07
mEq/L) and KO (1.15 ±0.14 mEq/L). Lithium treatment significantly
reduced body weight relative to control treatment (lithium WT weight change
relative to pre-drug: -11.8±1.6%; control WT change:
+1.8±0.9%; lithium KO: -10.9±2.5%;
control KO: +1.9±1.2%) (main effect of treatment:
F1,56=64.98, p<.01; main effect of genotype:
ns).Levels of phospho-MARCKS in prefrontal cortex (PFC) were significantly
higher in control-treated (t=3.49, df=10,
p<.01) but not lithium-treated KO relative to WT (Figure 7C). Levels of phospho-neuromodulin in
PFC were also significantly higher in control-treated (t=3.19,
df=10, p<.01) but not lithium-treated KO
relative to WT (Figure 7D). Genotypes did
not differ in striatal phospho-MARCKS (WT/control=1.0 ±0.1,
WT/lithium=1.2 ±0.4, KO/control=1.4 ±0.3,
KO/lithium=1.2 ±0.3) or phospho-neuromodulin
(WT/control=1.0 ±0.1, WT/lithium=0.8 ±0.1,
KO/control=1.0 ±0.1, KO/lithium=0.9 ±0.1).
Discussion
The goal of the current study was to test whether mutant mice lacking GluA1AMPAR subunit exhibit ‘mania-related’ phenotypic abnormalities.
Taken together with earlier studies demonstrating that GluA1 KO exhibit
schizophrenia- and depression-related phenotypes under certain conditions, the
current study suggests that these mice phenocopy features of schizoaffective
disorder.Replicating a phenotype consistently observed in our laboratories and
elsewhere (Bannerman et al., 2004; Chourbaji et al., 2008; Vekovischeva et al., 2004; Wiedholz et al., 2008), GluA1 KO showed a marked
hyperlocomotor response during exposure to a novel open field. Importantly, this is
a specific response to novelty rather than chronic elevation of locomotor activity,
because here and previously (Wiedholz et al.,
2008), we have shown that GluA1 KO display normal locomotion in the
familiar environment of the home cage. Thus, KO appear to be highly sensitive to the
stimulatory/provocative characteristics of a novel environment and, indeed, are slow
to habituate to such environments (Sanderson et al.,
2009). Extending these findings, current data show that open field
locomotor hyperactivity can also be provoked in GluA1 KO by exposure to even mild
stress. Following a single intraperitoneal saline injection, locomotor activity was
suppressed in WT but transiently increased above already elevated baseline levels in
GluA1 KO. Similarly, after 5 minute restraint, GluA1 KO again showed an exaggerated
short-lasting increase in open field locomotor activity. Collectively, these data
show that KO are highly sensitive to environmental provocation, and behaviorally
express this response in an open field setting with hyperactivity.GluA1 KO also showed a strong locomotor activity response (reduced
immobility) to the more intense stress of forced swim. As with the open field
locomotor hyperactivity phenotype, the forced swim phenotype was highly consistent
across different cohorts of mice and across laboratories. Of note, the response
diminished with repeated exposure, providing another indication that the
hyperactivity response in these mice is particularly strong to novel stimuli.
Moreover, a modified version of the test revealed that the reduced immobility was
the result of increased swimming behavior but not climbing. Given that reductions in
immobility due to increased swimming are produced by antidepressant treatments that
boost serotonin, rather than catecholamine, levels (Cryan et al., 2005), this phenotype could reflect a serotonin-related
antidepressant-like response (note, basal hippocampal serotonin levels are depressed
in GluA1 KO (Chourbaji et al., 2008)). Given
our open field data in KO, together with clinical data showing that stress
exacerbates psychomotor symptoms in bipolar disorder and schizophrenia (Ambelas, 1979; Malkoff-Schwartz et al., 2000), a more parsimonious interpretation is
that the forced swim behavior of these mice is a manifestation of a
‘manic-like’ hyperlocomotor response. Previous studies have
similarly interpreted this combination of behavioral abnormalities in other KOs
(e.g., Clock KO: Roybal et al., 2007; GluA6
KO: Shaltiel et al., 2008).Schizophrenia and bipolar disorder are often comorbid with anxiety
disorders, although bipolar disorder is more likely to be characterized by
risk-taking and novelty-seeking (DSM-IV,
1994). GluA1 KO showed increased entries into the open arms of the elevated
plus-maze and light compartment of the light/dark emergence test, as well as
consistent trends for increased time spent in these areas. This was another
phenotype that was remarkably stable across different laboratories and genetic
backgrounds (C57BL/6J and C57BL/6J×CBA/J hybrid), which is particularly
notable given evidence that the penetrance of mutant phenotypes in the elevated
plus-maze can vary with laboratory (Crabbe et al.,
1999) and background (Holmes and Hariri,
2003). Our data are also in general agreement with earlier work showing
increased light-compartment exploration and trends for increased open arm time
(Vekovischeva et al., 2004). Such
profiles are typically interpreted as a decrease in anxiety-like behavior.However, these anxiety tests are based upon a conflict between
threat-related avoidance and novelty-driven approach (Cryan and Holmes, 2005). In this context, data from other
tests and previous studies do not fit well with a decrease in anxiety-like behavior
in GluA1 KO and indicate a more complex phenotype. KO exhibited a profile in the
elevated zero-maze and stress-induced hyperthermia assays more consistent with
heightened anxiety-like behavior. It is conceivable that the greater increase in
core body temperature in KO could reflect increased muscle activity resulting from
stress-induced motor hyperactivity. Nevertheless, the profile in the zero-maze
resembles earlier data in the hyponeophagia and black/white alley tests (Bannerman et al., 2004). In addition, KO showed
a strong preference for the center of the elevated plus-maze and spent more time
scanning the light compartment, behaviors reflective of risk-assessment (Blanchard and Blanchard, 1989; Holmes and Rodgers, 1998). Thus, taken collectively and
with our findings in other tests, the profile in the plus-maze may reflect a
manic-like increase in approach-behavior perhaps related to heightened
‘novelty-seeking’ or ‘risk-taking.’ Clearly though,
additional experiments will be needed to fully understand the nature of this
phenotype. For example, it is not clear which facet of certain tests (plus-maze,
light/dark) brings out the KO approach-behavior that is not present in others
(zero-maze, black/white alley, hyponeophagia) where KO actually show less approach.
Of course the distribution of time spent in the different sections of these mazes
will, in part, reflect the relative ability of each section to induce exploration
which in turn will depend on the salience of the different sections, the starting
location of the mouse, and the rate of habituation in the different genotypes (Sanderson et al., 2009), resulting in a complex
set of interactions that could differ from one test to the next. Indeed, these data
underscore the complexity of these ostensibly simple mouse behavioral tasks that are
commonly employed, but not always carefully interpreted (Holmes, 2001).While the phenotype of locomotor hyperactivity and heightened-approach, at
least in certain tests, displayed by GluA1 KO models positive symptoms in
schizophrenia and the manic-like component of schizoaffective disorder, it also
resembles other neuropsychiatric disorders, including Attention Deficit
Hyperactivity Disorder (ADHD) (Brigman et al., in
press; Gainetdinov et al., 1999;
Powell and Miyakawa, 2006). For example,
dopamine transporter (DAT) KO also exhibit novelty-induced locomotor hyperactivity,
and this phenotype is normalized by psychostimulants that produce paradoxical
calming effects in persons with ADHD (Gainetdinov et
al., 1999). A model of bipolar mania or schizophrenia, by contrast, would
be expected to be worsened not rescued by psychostimulants, in line with the
response shown by schizophrenics and manicpersons. Consistent with this, and
arguing against an ADHD-like phenotype, acute treatment with the psychostimulant
anti-ADHD drugs, amphetamine (Adderall) and methylphenidate (Ritalin), exacerbated
rather than reversed open field hyperactivity in KO. One caveat here is these
effects were observed over a relatively short, 10 minute, test session, precluding a
fuller examination of the time course of genotype differences in psychostimulant
responsivity.Another set of important pharmacological findings was that two weeks of
treatment with the anti-manic drug, lithium, normalized the GluA1 phenotype in the
elevated plus-maze, although only partially in the novel open field. A similar
lithium treatment regimen normalized mania-related behavior in the elevated
plus-maze, but not novel open field, in Clock mutant mice (Roybal et al., 2007) (but not GluA6 KO, Shaltiel et al., 2008). The relative
insensitivity of the open field hyperactivity in GluA1 and Clock
mutants to lithium treatment may be a reflection of the relatively greater strength
of this phenotype. The GSK-3β inhibitor, SB216763, had weak but
non-significant reversing effects on the open field but not forced swim
hyperactivity phenotype of GluA1 KO. The GSK-3β pathway is a major target of
lithium (Gould and Manji, 2005) and SB216763
was recently shown to normalize open field and forced swim hyperactivity in DISC1
mutant mice (Mao et al., 2009). Additional
studies are warranted to further probe the GSK-3β pathway in GluA1 KO.
However, taken together, the main conclusion from these experiments is that
anti-manic drugs rescue at least a subset of the behavioral abnormalities in GluA1
KO. This extends our previous finding that haloperidol, an antipsychotic with
efficacy in schizophrenia and mania, also normalizes behavior (in that instance,
hyperlocomotion) in GluA1 KO (Wiedholz et al.,
2008). This pattern of pharmacological rescue further speaks to a KO
phenotype that may have features relevant to both mania and schizophrenia.In this context, the ability of lithium to rescue phenotypic abnormalities
in GluA1 KO was paralleled by normalization of elevated phosphorylation of MARCKS
and neuromodulin, two markers of the PKC pathway that interact with GluA1 and are
implicated in mania (Szabo et al., 2009).
These molecular abnormalities and their reversal by lithium were seen in PFC but not
striatum, suggesting the primary PKC alteration was at the cortical level. This
raises the possibility that the increased plus-maze approach phenotype in KO is
driven by PFC dysfunction (although note that excitotoxic PFC lesions do not
typically affect this behavior: Holmes and Wellman,
2009; Rudebeck et al., 2007),
while the novelty-induced hyperactivity phenotype may occur independently of frontal
regions. It has been suggested that the open field hyperactivity in these mice has a
striatal and dopaminergic basis because of our previous finding of reduced striatal
dopamine clearance and aforementioned phenotypic rescue by haloperidol (a dopamine
D2 receptor antagonist) (Wiedholz et al.,
2008). On the other hand, a surprising finding from the current study was
that rapid depletion of dopamine via AMPT treatment did not reverse open field
hyperactivity in GluA1 KO (as it does in DAT KO: Costa et al., 2006; Gainetdinov et al.,
1999), but actually exacerbated the phenotype despite effectively
depleting striatal dopamine tissue levels. The reasons for this paradoxical response
are unclear and require further study.The study of constitutive GluA1 KO does not allow us to distinguish between
effects of GluA1 absence just during adulthood and consequences arising from
developmental disturbances. Of note in this context, a recent microarray analysis
revealed multiple changes in the hippocampal expression of calcium signaling
proteins in GluA1 KO (Zhou et al., 2009).
Although we found that non-mutant C57BL/6J mice systemically treated with the
subunit-non-selective competitive AMPAR antagonist, GYKI 52466, did not show KO-like
hyperactivity or approach behavior this cannot be readily equated with the complete,
subunit-specific nature of the GluA1 KO. Notwithstanding, we cannot exclude the
possibility that the mania-related phenotype in GluA1 KO is the consequence of a
complex set of changes in glutamate neurotransmission as well as ontogenic insults
in, for example, corticostriatal wiring. This would not, however, lessen the
potential validity of the mutant as a model of a human affective or psychotic
disorder, which are themselves posited to have a major developmental etiological
component (Hariri and Holmes, 2006; Harrison and Weinberger, 2005). Another
potential issue that was not fully addressed in the current study is the possible
modifying influence of sex on the GluA1 phenotype. We had previously found no
evidence that male and female GluA1 KO differed on various phenotypic measures,
including schizophrenia- and fear related behaviors (Feyder et al., 2007; Wiedholz et al.,
2008) and therefore did not design or power the current study to address
sex as an interacting factor. We therefore cannot wholly discount a possible sex
influence on the current measures, and this remains another interesting question for
future studies in these mutants.In summary, the current study demonstrates that KO of GluA1 produces a
profound and selective increase in locomotor activity in response to novelty, and
mild and intense stressors. GluA1 KO displayed a complex profile in tests for
anxiety-like behavior, with an increased (novelty-seeking or risk-taking related)
approach drive in some, but not all, tests. At least some of these behavioral
abnormalities were normalized by the anti-manic drug lithium, but were aggravated
further by psychostimulants and by rapid dopamine depletion. GluA1 KO and increased
approach behaviors were associated with increased PKC activity in PFC. Taken
together with previous studies showing these mice exhibit schizophrenia- and
depression-related abnormalities, we propose that these mice may phenocopy features
of schizoaffective disorder and provide a novel tool for studying the
pathophysiology of this disorder.
Authors: G Shaltiel; S Maeng; O Malkesman; B Pearson; R J Schloesser; T Tragon; M Rogawski; M Gasior; D Luckenbaugh; G Chen; H K Manji Journal: Mol Psychiatry Date: 2008-03-11 Impact factor: 15.992
Authors: Yingwei Mao; Xuecai Ge; Christopher L Frank; Jon M Madison; Angela N Koehler; Mary Kathryn Doud; Carlos Tassa; Erin M Berry; Takahiro Soda; Karun K Singh; Travis Biechele; Tracey L Petryshen; Randall T Moon; Stephen J Haggarty; Li-Huei Tsai Journal: Cell Date: 2009-03-20 Impact factor: 41.582
Authors: David J Sanderson; Mark A Good; Kathryn Skelton; Rolf Sprengel; Peter H Seeburg; J Nicholas P Rawlins; David M Bannerman Journal: Learn Mem Date: 2009-05-23 Impact factor: 2.460
Authors: Kole Roybal; David Theobold; Ami Graham; Jennifer A DiNieri; Scott J Russo; Vaishnav Krishnan; Sumana Chakravarty; Joseph Peevey; Nathan Oehrlein; Shari Birnbaum; Martha H Vitaterna; Paul Orsulak; Joseph S Takahashi; Eric J Nestler; William A Carlezon; Colleen A McClung Journal: Proc Natl Acad Sci U S A Date: 2007-03-22 Impact factor: 11.205
Authors: Peter H Rudebeck; Mark E Walton; Benjamin H P Millette; Elizabeth Shirley; Matthew F S Rushworth; David M Bannerman Journal: Eur J Neurosci Date: 2007-10-10 Impact factor: 3.386
Authors: Won Sub Kang; Jin Kyung Park; Su Kang Kim; Hae Jeong Park; Sang Min Lee; Ji Young Song; Joo-Ho Chung; Jong Woo Kim Journal: Mol Biol Rep Date: 2012-10-08 Impact factor: 2.316
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