Neocortical Long-Term Potentiation and Experience-Dependent Synaptic Plasticity Require {alpha}-Calcium/Calmodulin-Dependent Protein Kinase II Autophosphorylation

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The Journal of Neuroscience, June 1, 2003, 23(11):4428-4436

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Neocortical Long-Term Potentiation and Experience-Dependent Synaptic Plasticity Require ${alpha}$ -Calcium/Calmodulin-Dependent Protein Kinase II Autophosphorylation
Neil Hardingham,¹^* Stanislaw Glazewski,¹^* Pavel Pakhotin,¹^* Keiko Mizuno,² Paul F. Chapman,¹ K. Peter Giese,² and Kevin Fox¹
¹ School of Biosciences, Cardiff University, Cardiff CF10 3US, United Kingdom, and ² Wolfson Institute for Biomedical Research, University College London, London WC1E 6BT, United Kingdom

   Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Experience-dependent plasticity can be induced in the barrelcortex by removing all but one whisker, leading to potentiationof the neuronal response to the spared whisker. To determinewhether this form of potentiation depends on synaptic plasticity,we studied long-term potentiation (LTP) and sensory-evokedpotentials in the barrel cortex of ${alpha}$ -calcium/calmodulin-dependentprotein kinase II ( ${alpha}$ CaMKII)^T286A mutant mice. We studied threedifferent forms of LTP induction: theta-burst stimulation,spike pairing, and postsynaptic depolarization paired withlow-frequency presynaptic stimulation. None of these protocolsproduced LTP in ${alpha}$ CaMKII^T286A mutant mice, although all threewere successful in wild-type mice. To study synaptic plasticityin vivo, we measured sensory-evoked potentials in the barrelcortex and found that single-whisker experience selectivelypotentiated synaptic responses evoked by sensory stimulationof the spared whisker in wild types but not in ${alpha}$ CaMKII^T286Amice. These results demonstrate that ${alpha}$ CaMKII autophosphorylationis required for synaptic plasticity in the neocortex, whetherinduced by a variety of LTP induction paradigms or by manipulationof sensory experience, thereby strengthening the case that the two forms of plasticity are related.

Key words: barrels; whiskers; LTP; mouse; synapse; plasticity

   Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Sensory experience can have a profound effect on neurons inthe neocortex. In the auditory cortex, experience alters thewidth of receptive field tuning (Kilgard et al., 2001), whereasin the visual cortex, cells are able to alter their occular-dominance and orientation tuning during a critical period of development (Blakemore and Cooper, 1970; Hubel and Wiesel, 1970). In thesomatosensory cortex, cells are able to alter their responsesto stimulation of specific digits or whiskers, both duringdevelopment and into adulthood (Simons and Land, 1987; Wall,1988; Glazewski and Fox, 1996). These experience-dependentchanges have been measured by observing spike firing rate butprobably rely on the underlying synaptic plasticity of the cortical excitatory neurons. Evidence to support this idea comesfrom experiments showing that ${alpha}$ -calcium/calmodulin-dependentprotein kinase II ( ${alpha}$ CaMKII) and ${alpha}$ CaMKII autophosphorylation isrequired for experience-dependent plasticity (Glazewski etal., 1996, 2000; Gordon et al., 1996; Taha et al., 2002)as well as synaptic plasticity (Silva et al., 1992; Gieseet al., 1998).
However, studies showing that ${alpha}$ CaMKII autophosphorylation isrequired for experience-dependent plasticity in the neocortexare thus far only based on recordings from sensory-evoked extracellularaction potentials (Glazewski et al., 2000; Taha et al., 2002). Theoretically, ${alpha}$ CaMKII autophosphorylation could affect spikeactivity by altering membrane potential, spike threshold, oraccommodation, or affect coupling of synaptic potentials withsomatic potentials by altering dendritic voltage-gated channels,all without directly affecting synaptic plasticity. Similarly,evidence that ${alpha}$ CaMKII autophosphorylation plays a role in synapticplasticity is based on recordings in the Schaeffer collateral–CA1pathway in the hippocampus (Giese et al., 1998), and it isnot known whether plasticity mechanisms are identical betweenneocortical pathways and the Schaeffer collateral–CA1pathway. Indeed, even hippocampal pathways differ in theirrequirement for CaMKII autophosphorylation (Errington et al., 2002).
Therefore, to test whether neocortical synaptic plasticity underlies neocortical experience-dependent plasticity, we undertook twotypes of experiments in the barrel cortex. First, we testedthe idea that long-term potentiation (LTP) in the barrel cortexmight depend on ${alpha}$ CaMKII autophosphorylation, using ${alpha}$ CaMKII^T286Apoint mutant mice (Giese et al., 1998). We studied three differentLTP induction paradigms, because it was not clear which paradigmmight be most relevant to the natural plasticity induction processes in the barrel cortex. We studied the pathway fromlayer IV to layer II/III of the near neighboring barrel becausethis was the most direct pathway that could be involved inthe in vivo plasticity, although not the only one (Fox, 2002).Second, we used current source density analysis to measurechanges in sensory-evoked dendritic currents associated withexperience-dependent plasticity in the barrel cortex. In thisway, we were able to measure changes more closely related tosensory-evoked synaptic potentials than was able to be achieved previously with spike recording. Third, we tested whether experience-dependent plasticity was dependent on ${alpha}$ CaMKII autophosphorylation in thecortex. The results demonstrate that both LTP and experience-dependentplasticity require ${alpha}$ CaMKII autophosphorylation in the barrelcortex and suggest that synaptic plasticity at excitatory pathwaysplays a major role in the expression of experience-dependentplasticity.

   Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Subjects. For Western blot analysis, subjects were three wild-type and three mutant mice. For LTP studies, subjects were male andfemale mice that were 4–6 weeks of age. A group of 30wild types and 28 mutants yielded 46 wild-type slices of barrelcortex and 62 slices from the mutants. All animals were studiedblind to the genotype.
For current source density studies, subjects were male and femalemice, 3–5 months of age. A group of 35 animals was used,including 10 deprived and 7 normally reared homozygotes and11 deprived and 7 normally reared wild types. All recordingswere done blind to the genotype. Animals were genotyped byPCR as described previously (Giese et al., 1998). The animalsstudied were the F₃ and F₄ generations of mice in which theoriginal generation was of a hybrid 129/Sv x C57BL/6 background.Only heterozygotes were bred (cousin matings).
Western blot analysis. Brain tissues from the somatosensorycortex and hippocampus were isolated from adult mice. Proteinextracts were prepared using 2% SDS, and the protein concentrationswere determined with the BCA assay (Pierce, Rockford, IL).Ten micrograms of each sample were separated on 4–15%SDS-PAGE (Bio-Rad, Hercules, CA) and transferred onto polyvinylidenedifluoride membranes (Bio-Rad). Antibodies against ${alpha}$ CaMKII (monoclonalantibody 6G9; Chemicon, Temecula, CA), ${beta}$ -actin (Clone AC-15;Sigma, St. Louis, MO), and synaptotagmin (rabbit; Sigma) were used. After incubation with a peroxidase-conjugated antibody(Pierce), immunoreactive bands were visualized using a chemiluminescentreagent (SuperSignal West Pico Chemiluminescent Substrate;Pierce) and analyzed by Quantity One (Bio-Rad). After visualization,membranes were washed in stripping buffer (Restore WesternBlot Stripping Buffer; Bio-Rad) and reused.
Electrodes and solutions for in vitro recording. In differentexperiments, field recording, current clamp, and voltage clampwere used. In all cases, the stimulating electrode was placedaccurately within the wall of a layer IV barrel under visualguidance using an Olympus Optical (Tokyo, Japan) BH2 videomicroscope and a transilluminated slice. For extracellularrecording, the recording electrode was positioned in the middle of layers II/III on the nearside of the adjacent barrel column.For intracellular recording, cells were chosen within thatsame area and patched under visual guidance using a 40x waterimmersion objective, differential interference contrast optics,and infrared illumination.
Slices were produced by conventional means. The slices weremaintained in a submersion chamber continually perfused (2–3ml/min) with artificial CSF containing (in mM): 119 NaCl, 3.5KCl, 1 NaH₂PO₄, 2 CaCl₂, 1 MgSO₄, 26 NaHCO₃, and 10 glucose.The solution was bubbled with 5% CO₂–95% O₂ and keptat room temperature (21–24°C). The extracellularrecording electrode was a carbon fiber microelectrode withthe tip etched to 25–40 µm. The intracellular electrodeswere 7–10 M ${Omega}$ and filled with (in mM): 110 K-gluconate,10 KCl, 2 MgCl₂, 2 Na₂ATP, 0.03 Na₂GTP, 10 HEPES, pH 7.3, and270 mOsm.
In vitro recording and LTP induction protocols. Whole-cell recordings of synaptic responses in layer II/III pyramidal neuronswere taken at the postbreak in resting membrane potential (mean± SD, 69 ± 4 mV) for current-clamp experimentsand at -65 mV for the voltage-clamp experiments. Series resistancewas monitored, and the recording was discarded if it changedby >20% during the course of the experiment. Monosynaptic components of the EPSPs or EPSCs were monitored and found tohave reversal potentials close to 0 mV for wild types (mean± SD, 1.8 ± 12.3 mV) and T286A mutants (4.8 ±9 mV), which were not different (t₍₁₉₎ = 0.38; p > 0.5).
Theta-burst stimulation consisted of groups of four 200 µseccurrent pulses at 100 Hz repeated at 5 Hz for 10 cycles asdescribed previously (Kirkwood et al., 1993). Field EPSPswere measured in responses to low-frequency (1 per 20 sec) stimulation, low-pass filtered at 10 kHz, and recorded using custom programsgenerated with LabVIEW software (National Instruments, AustinTX).
Two pairing protocols were used. In both cases, the presynapticstimulation rate was increased to 2 Hz. With depolarizationpairing, current was injected to move the cell to a positivepotential ( $~$ 0 mV) for 1 min. With spike pairing, a brief 10msec current pulse was injected, sufficient to produce a postsynapticspike at the end of the naturally evoked EPSP. The interval between presynaptic and postsynaptic spikes was therefore controlledat 10 msec, and the condition was repeated 120 times.
Whisker deprivation. To induce plasticity, the D1 vibrissa was spared for 18 d, whereas all surrounding vibrissas were deprivedevery second day. Deprived vibrissas were allowed to regrowfor 8–10 d before the recording session. The deprivationtechnique used was found to not affect vibrissa innervation(Li et al., 1995) and has been described in detail previously (Glazewski et al., 1998).
Anesthesia and surgery. Anesthesia was induced with fluothane (Zeneca, Cheshire, UK) and maintained with intraperitoneal injectionsof urethane (1.5 gm/kg whole body weight; Sigma). Depth ofanesthesia was monitored by testing hindlimb reflexes and monitoringthe EEG. Animals were reinjected with 10% of the initial doseof urethane if the hindlimb reflex was brisk. The skull overlyingthe barrel cortex was thinned by careful drilling. A smallhole just large enough for the electrode to pass through wasmade in the skull before each electrode penetration using ahypodermic needle. All experiments complied with the UnitedKingdom Animals (Scientific Procedures) Act of 1986.
Electrodes, stimulus, and recording. Glass-insulated carbonfiber microelectrodes were used to record from the cortex (Armstrong-James et al., 1980). Vibrissas were stimulated at0.1 Hz using a computer-controlled piezoelectric stimulatordriven by a voltage source (DS-2; Digitimer, Welwyn Garden,UK). All recordings were made from layers II–V. Usuallyone electrode penetration was made per animal. The neuronswere sampled every 50 µm through the depth of the penetration(-50 to 700 µm). Ten waveforms were averaged for eachrecording site. Principal and intact (D1) whiskers and one surround-deprived whisker were stimulated at each depth. Afteradvancing the electrode 50 µm, a 10 min pause enabledthe recording to stabilize. The stimulus intensity was normalizedby adjusting it to 50–60% of the maximal principal whiskerresponse within layer IV (300 µm below the pia) and waskept constant afterward throughout the penetration. The testpulse was generated using Spike2 software (Cambridge ElectronicDesign, Cambridge, UK). Field potentials [sensory-evoked potentials(SEPs)] were recorded using the Neurolog system (Digitimer)and filtered between 0.1 and 1.5 kHz without a 50 Hz notchfilter. Waveforms were amplified 500 times and digitized. Waveforms were monitored, acquired, and averaged using in-house programswritten in LabVIEW software (National Instruments).
Current source density analysis. Current source density (CSD)was calculated using methods described previously (Mitzdorfand Singer, 1978; Mitzdorf, 1985) from averaged field potentialsas follows:

where i_x and V_x are thecurrent and voltage at depth x µm below the pial surface, V_{x - 50} is the depth 50 µm above depth x, and ${sigma}$ is thevolume conductance. Gray-scale images of the CSD profiles weremade using NIH Image as described previously (Aizenman et al.,1996). The maximum and minimum of the scale were determinedby the largest peak current recorded in this series of experimentsand were symmetrical at $~$ 0. The maximum layer II/III sink resultingfrom "spared" whisker stimulation was identified for each penetrationand the spared- and principal-whisker SEPs analyzed for thatdepth.
Histology. After every experiment, the animal was deeply anesthetizedwith urethane and perfused through the heart with 100 mM PBS,followed by PBS containing 4% paraformaldehyde and increasingconcentrations of sucrose. The brain was removed and the cortexwas flattened, as described previously (Strominger and Woolsey, 1987), and left overnight in 20% sucrose in buffered solutionof formaldehyde. Sections of 40 µm were cut tangentiallyto the surface of flattened cortex and the tissue reacted forcytochrome oxidase (Wong-Riley, 1979). Recording locationswere identified from focal lesions (1 µA, 10 sec; tipnegative) made at the end of each penetration within the cytochromeoxidase-stained sections of the barrel field.
Statistical analysis. For the in vitro experiments, individualtime-course recordings were normalized and averaged within groups as a series of 10 min epochs. ANOVAs were used to test for effectsof and interactions between genotype, time, and tetanus protocol.Post hoc repeated-measures t tests were used to find the sourceof effects and interaction terms.
For the in vivo experiments, the ratio of spared and principal whisker response was calculated for each penetration. Populationaverages were calculated for spared whisker response, principalwhisker response, and the ratio of the two. The averages ofthese populations were analyzed by ANOVA and, where applicable,post hoc t tests were used.

   Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

${alpha}$ CaMKII protein levels in the somatosensory cortex of ${alpha}$ CaMKII^T286A mice
Recent studies have shown that ${alpha}$ CaMKII levels are reduced inthe visual cortex of ${alpha}$ CaMKII^T286A point mutants (Taha et al.,2002). Therefore, we measured ${alpha}$ CaMKII protein levels in thesomatosensory cortex and hippocampus of the same animals. Theexpression of ${alpha}$ CaMKII in mutants and wild types was normalizedto the expression of ${beta}$ -actin in each animal to minimize errorsin protein loading and transfer (Fig. 1). In somatosensory cortex, ${alpha}$ CaMKII expression was significantly reduced by 25% inthe mutants (F_(1,4) = 13.7; p < 0.05). In contrast, thelevels of ${alpha}$ CaMKII in the hippocampus of the same mutant micewere not different from those in wild types (F_(1,4) = 0.002;p = 0.96). Therefore, the results show that ${alpha}$ CaMKII levels areslightly reduced in a region-specific manner in the cortex of ${alpha}$ CaMKII^T286A point mutant mice.

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Figure 1. Immunoblot analysis of ${alpha}$ CaMKII expression in the somatosensory cortex (Sm Cx) and hippocampus (Hi) in ${alpha}$ CaMKII ^T286A mutants (T286A; n = 3) and wild-type littermates (wt; n = 3). The samples from three mutants (t286A-1, t286A-2, and t286A-3) and three wild-type littermates (wt-1, wt-2, and wt-3) are shown. A, The immunoblots were used first for detecting ${alpha}$ CaMKII expression, and, after stripping of the blots, ${beta}$ -actin expression was determined as a standard for normalization. B, Expression in the somatosensory cortex was quantified and plotted in reference to expression in wild-type littermates (white bars). There was only a trend to suggest that ${alpha}$ CaMKII expression was reduced in the mutants (F_(1,4) = 6.29; p = 0.066), whereas ${alpha}$ CaMKII expression normalized to ${beta}$ -actin expression was significantly reduced by 25% (F_(1,4) = 13.7; p < 0.05) C, Expression in the hippocampus was quantified and plotted in reference to expression in wild-type littermates (white bars). The ${alpha}$ CaMKII expression in the mutants was significantly reduced by 17% (F_(1,4) = 9.09; p < 0.05), but this reduction could not be confirmed when the ${alpha}$ CaMKII expression was normalized to ${beta}$ -actin expression (F_(1,4) = 0.002; p = 0.96). Error bars depict SEMs.

${alpha}$ CaMKII autophosphorylation is required for theta-burst-induced cortical LTP
To study the role of ${alpha}$ CaMKII autophosphorylation in corticalLTP, we recorded extracellular field potentials in layers II/IIIof the barrel cortex in slices prepared from the ${alpha}$ CaMKII^T286Amice and their wild-type littermates. To compare our resultswith previous studies, we used a theta-burst stimulation protocol,which has been shown previously to induce NMDA-dependent LTPin visual cortex (Kirkwood et al., 1993). When the stimulatingelectrodes were placed in the wall of the barrel under visual guidance and the recording electrode in layers II/III of theneighboring barrel (see Materials and Methods), we were ableto evoke LTP (of at least 15%) in all slices derived from wild-typemice.
To test whether the method evoked NMDA-dependent LTP in thebarrel cortex, we applied 25 µM D-AP-5 to the slice 10min before theta-burst stimulation. The peak did not increasesignificantly above baseline after tetanus (Fig. 2A) (average± SEM, 104.9 ± 2.5%; p > 0.07; n = 10; t test).In contrast, a second tetanus applied to the same slices 1hr after the washout produced LTP that persisted for at least1 additional hour (Fig. 2A) (121.3 ± 5.8%; p < 0.02;n = 10; t test). This result shows that theta-burst stimulationproduces NMDA-receptor-dependent LTP in the layer IV to II/IIIpathway between columns in the barrel cortex.

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Figure 2. Dependence of barrel cortex LTP on NMDA receptors and ${alpha}$ CaMKII autophosphorylation. A, Time plots of average extracellular field potentials evoked in the middle of layer II/III by stimulation of layer IV in the nearside barrel. Theta-burst tetanization (leftmost arrow) in the presence of 25 µM D-AP-5 did not induce potentiation. However, when the AP-5 was washed out of the bath and a second tetanus was presented (rightmost arrow), LTP was induced and lasted for at least 1 hr. The dashed line indicates the baseline 15 min before the first (100%) and second (104%) tetanus. B, Theta-burst stimulation was applied (arrow) to slices derived from ${alpha}$ CaMKII ^T286A mice (black circles) or their wild-type littermates (white circles). LTP was not induced in the mutants but was induced in the wild-type mice. EPSP peaks are shown for each stimulus once every 20 sec. Error bars are SEs calculated for the preceding 1 min. fEPSP, Field EPSP.

To see whether this form of LTP was also dependent on ${alpha}$ CaMKII autophosphorylation, we applied the same protocol to barrelcortical slices prepared from 15 homozygous ${alpha}$ CaMKII^T286A miceand 10 wild-type littermates. The mutation prevented LTP, ascan be seen in Figure 2B. The response increased to 126.4± 6.1% of baseline at 1 hr in wild-type mice but only104.4 ± 4.5% in the mutants. Analysis revealed a significantmain effect of time (F_(6,14) = 7.76; p < 0.0005) and genotype(F_(1,19) = 14.73; p < 0.002) and an interaction betweentime and genotype (F_(6,14) = 4.41; p < 0.02). Post hoc tests showed that all time points were significantly differentbetween genotypes except for the first two 10 min epochs aftertetanization, indicating that LTP induced by theta-burst stimulirises slowly in the wild types and not at all in the mutants.In five mutants and four wild-type mice, LTP was followed for1 additional hour. The degree of potentiation was equivalentat 2 hr to that shown at 1 hr in the wild-type mice (140.9 ± 4.9%), whereas no LTP was seen at all in the mutants (91.1 ±8.2%; data not shown). In conclusion, LTP induced by theta-burststimulation requires ${alpha}$ CaMKII autophosphorylation in layers II/IIIof the neocortex.
${alpha}$ CaMKII is required for pairing-induced LTP
After pretetanus baseline recording (at the resting membranepotential), LTP was induced by injecting sufficient currentto depolarize the cell to $~$ 0 mV for 1 min while delivering afferentpresynaptic stimulation at 2 Hz (depolarization protocol) orby injecting a brief 10 msec current pulse sufficient to inducea postsynaptic action potential directly after the presynapticstimulus (spike-pairing protocol). Postsynaptic spikes wereabsent with the depolarization protocol and present with thespike-pairing protocol.
The T286A mutation was again found to prevent LTP, whether inducedby spike pairing or the depolarization protocol. Statisticalanalysis revealed an effect of genotype (F_(1,35) = 9.02; p< 0.005) but not of the stimulation protocol (i.e., spikepairing vs depolarization pairing) (F_(1,35) = 1.81; p <0.19) nor any interaction between the two (F_(1,35) = 0.29;p = 0.59). We also found an interaction of time and genotype (F_(6,30) = 2.49; p < 0.05). As can be seen in Figure 3,this interaction is probably caused by the faster decay ofthe potentiated state in the ${alpha}$ CaMKII^T286A mice compared withwild-type mice. Post hoc tests showed that whereas the wild-typeEPSPs remained potentiated at 60 min, the EPSPs decayed backto baseline after 20 min in the mutants (Fig. 3).

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Figure 3. The effect of ${alpha}$ CaMKII autophosphorylation on pairing-induced potentiation of cortical EPSPs. Top, Example traces are shown of EPSPs (average of 10 responses) recorded before and after depolarization pairing for cells recorded from a wild-type and ${alpha}$ CaMKII ^T286A homozygote mouse. Immediately after induction, both genotypes show potentiation (0–10 min; middle traces), but only the wild type shows potentiation at 60 min in this case (right traces). Calibration: 2 mV, 50 msec. Bottom, The normalized peak EPSP amplitude is averaged across cells and plotted against time for layer II/III pyramidal cells in response to stimulation of the nearside edge of the layer IV barrel. Averaged normalized EPSPs are represented for 20 cells in the mutants and nine cells in the wild types. Although pairing depolarization with 2 Hz of presynaptic stimulation or pairing a postsynaptic spike 10 msec after the presynaptic stimulus (arrow) induced rapid potentiation in both wild types (white circles) and ${alpha}$ CaMKII ^T286A mutants (black circles), the potentiation decayed in the mutants with in 20 min, where as in the wild types, potentiation was present for at least 1 hr. The dashed line indicates the baseline 15 min before tetanus (100%). Error bars are SE calculated for the preceding 2 min.

Similar results were found in cases in which EPSCs were measured.Layer IV stimulation evoked EPSCs that were recorded in layerII/III cells at a holding potential close to -65 mV. Sustaineddepolarization to 0 mV for 1 min during 1 Hz presynaptic stimulationproduced LTP in wild types but potentiation that decayed tobaseline by 40 min in the mutants (Fig. 4). Statistical analysis showed an effect of genotype (F_(1,49) = 23.55; p < 0.0001)and time (F_(4,46) = 1.73; p < 0.0001) and an interactionbetween the two factors (F_(4,46) = 0.65; p < 0.0001). Posthoc t tests showed that this was because the wild types potentiatedat all times after pairing, whereas the ${alpha}$ CaMKII^T286A mice showed potentiation at 30 min but not at 40 min after pairing.

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Figure 4. The effect of ${alpha}$ CaMKII autophosphorylation on pairing-induced potentiation of cortical EPSCs. Top, Example traces of EPSCs recorded before and 40 min after pairing presynaptic and postsynaptic depolarization for 1 min in a wild-type and an ${alpha}$ CaMKII ^T286A homozygote mouse. Calibration: 100 pA, 10 msec. Bottom, Averaged normalized EPSCs recorded from 31 cells in wild types (white circles) and 31 cells in CaMKII ^T286A homozygotes (black circles). Pairing presynaptic stimulation at 1 Hz with constant depolarization causes sustained potentiation in wild-type neurons; EPSCs show a slowly decaying level of potentiation that is statistically indistinguishable from baseline at 40 min. The dashed line indicates the baseline 10 min before tetanus (100%). Error bars are SE calculated for the preceding 2–5 min.

These results demonstrate a fundamental deficit in the mechanismsof LTP induction in ${alpha}$ CaMKII^T286A mice that is independent oftetanus protocol or whether field EPSPs, EPSPs, or EPSCs aremeasured (Fig. 5).

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Figure 5. Comparison of the effect of LTP induction protocol and genotype on potentiation. LTP induced by theta-burst potentiation ( ${theta}$ -burst) produced levels of potentiation equivalent to those obtained by spike pairing and depolarization pairing (Depol. pairing) protocols in wild-type mice (white bars). Potentiation was greater in voltage-clamped neurons than in the other cases (141 vs 121–126%). In contrast, none of the four protocols produced LTP in the ${alpha}$ CaMKII^T286A mutants. The bars represent averages taken between 50–60 min after tetanus or pairing, except for the EPSCs, which are measured at 30–40 min after pairing. fEPSP, Field EPSP. Error bars represent SEs.

Whisker deprivation causes potentiation of sensory-evoked potentials
To test whether SEPs are enhanced in the barrel cortex of wild-typemice after whisker stimulation, we stimulated a single whiskerwhile recording the SEP at a known depth within the cortex (Fig. 6). By averaging SEPs at each depth and measuring themevery 50 µm, it was possible to construct a CSD profileof SEPs and currents within an electrode penetration betweenthe cortical surface and layer V. The maximum amplitude ofthe CSDs decreased as a function of distance from the principalbarrel of the stimulated whisker. We therefore compared CSDsin deprived and undeprived mice at similar distances from thebarrel of the spared whisker (Fig. 7). The distances were measuredfrom microlesions made at the end of recording in each penetrationvisualized in the cytochrome oxidase histology of the barrelfield. Even without normalizing the currents across animals,it was clear from the CSD profiles that larger currents wereevoked by the spared whisker after a period of 18 d of single-whiskerexperience compared with currents evoked by the same whiskerin undeprived animals. We found that currents were greaterin all layers after deprivation. The earliest currents afterstimulation of the spared whisker occurred in layers II/III, followed by layer IV and V.

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Figure 6. The effect of whisker deprivation on SEPs in the barrel cortex of wild-type (WT) and homozygous ${alpha}$ CaMKII ^T286A mice. Left column, SEPs were recorded in the D2 barrel-column for a rapid deflection of the D2 whisker (dashed line) or the D1 whisker (solid line). In a normal animal, the amplitude of the potential is smaller for the surround receptive-field whisker (D1 in this case) than for the principal whisker (D2 in this case) at most depths. Middle column, Whisker deprivation increases the amplitude of the spared whisker SEPs so that they were at least as great as those evoked by the principal whisker. Right column, Despite a period of single-whisker experience, the spared (D1) whisker (solid line) shows a far smaller response than the principal whisker in homozygous ${alpha}$ CaMKII ^T286A mice (dashed line). Calibration: 3 mV, 50 msec. Note that the potentials at intermediate depths are not shown for clarity (i.e., those at -50, 50, 150 µm, etc.).

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Figure 7. CSD analysis of SEPs in wild-type mice. CSD is plotted for penetrations made in the barrel neighboring D1. Currents were evoked by stimulating the D1 whisker and calculated from field potentials measured every 50 µm. Responses are normalized across all cases and plotted on a gray scale in which the maximum sink is represented by white, the maximum source by black, and zero by mid-gray. Examples are shown at various distances from the D1 barrel penetration as indicated by the insets, in which the white circle represents the location of the penetration. Top row, The earliest sink can be seen in superficial layers and later in layer IV in animals deprived of all but the D1 whisker. The amplitude of the sinks and sources decreases with distance from the D1 barrel. Bottom row, The equivalent CSD analysis in animals that have not undergone whisker deprivation. Cases were taken for identical D1 stimulation at distances from the D1 barrel matched as closely as possible to those shown on the top row. The sinks and sources evoked by D1 stimulation were far weaker in undeprived animals.

${alpha}$ CaMKII autophosphorylation is necessary for potentiation of SEPs
To test whether ${alpha}$ CaMKII autophosphorylation was required for potentiation of SEPs, we repeated the deprivation study in homozygous ${alpha}$ CaMKII^T286A mice and their wild-type littermates. The CSD profilesindicated a lack of plasticity in the mutants, because theywere unchanged between the deprived and undeprived mutant animals (Fig. 8). To quantify the data, we identified the locus ofthe largest superficial layer II/III sink for each penetrationand compared the SEP amplitude for the principal whisker (which was always a deprived whisker for the deprived mice) for eachpenetration and the spared whisker (Fig. 6).

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Figure 8. Whisker-deprivation plasticity depends on autophosphorylation of ${alpha}$ CaMKII as assessed by CSD analysis. CSD is plotted on a gray scale as described in Figure 7. The sinks (white) and sources (black) evoked by stimulating the spared whisker (D1) were weak in both deprived and undeprived ${alpha}$ CaMKII ^T286A mutants. Penetrations were chosen for matched distances from the D1 barrel. The insets show the position of the penetration relative to the D1 barrel (white circle). Top row, Deprived animals. Bottom row, Undeprived animals.

In wild-type mice, the spared-whisker SEP increased to the sameamplitude or greater than the principal-whisker SEP. The increasein the ratio of spared-whisker to principal-whisker SEP, from0.45 to 1.64 (averaged across the barrel neighboring the sparedbarrel), in the wild-type mice did not occur in the ${alpha}$ CaMKII^T286Amice (0.60 in undeprived mice vs 0.74 in deprived mice). Statisticalanalysis showed that the ratio of the spared-to the principal-whiskerresponse was affected by deprivation (F_(1,33) = 2.9; p <0.0005) and by genotype (F_(1,33) = 4.5; p < 0.05), and thatthere was an interaction between genotype and deprivation (F_(1,33)= 1.8; p < 0.005). The interaction was caused by an increasein the spared-whisker-evoked SEPs that was not observed inthe ${alpha}$ CaMKII^T286A animals (Fig. 9). These findings thereforeshow that experience-dependent synaptic potentiation normallyoccurs in the mouse barrel cortex, and that this plasticityrequires autophosphorylation of ${alpha}$ CaMKII.

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Figure 9. Quantification of SEPs as a function of distance from the principal barrel of the spared whisker. The ratio of the spared to principal whisker sensory-evoked potentials is plotted as a function of distance from the edge of the barrel of the spared whisker. Each point represents a ratio of time-averaged responses for the maximum layer II/III sink in each penetration. The black bar beneath the x-axis indicates the approximate extents of the neighboring barrel. Top left, In undeprived wild-type mice, the ratio decreases with increasing distance from the D1 barrel. The average ratio of the D1 to the principal whisker-evoked potential between 50 and 250 µm from the edge of the D1 barrel is shown by the horizontal dashed line. Top right, After a period of single-whisker experience, the spared whisker evoked a far greater response in the neighboring barrel. Bottom left, Response ratios decreased with distance from the D1 barrel in homozygous ${alpha}$ CaMKII ^T286A mice, just as in wild-type mice. Bottom right, A period of single-whisker experience does not lead to an increase in the ratio of the D1 to principal whisker response in the mutants.

   Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The relationship between an artificially induced synaptic plasticity mechanism such as LTP and naturally induced potentiation isnot easy to prove. The advantage of studying the relationshipin the somatosensory cortex is that the form of potentiationis very similar in the two cases. Sensory-evoked potentialsare enhanced in layer II/III of the neighboring cortical column after single-whisker experience, and a similar form of potentiationcan be induced by theta-burst stimulation in the IV to II/IIIpathway between columns in slices (this study) or in vivo (Glazewski et al., 1998). From a conservative viewpoint, wecan only say that we have not disproved that the two phenomenaare different. However, LTP and experience-dependent potentiationdo show a remarkably detailed level of dependence on the same synaptic mechanism, even to the level of requiring the same ${alpha}$ CaMKII phosphorylation state.
We found that total ${alpha}$ CaMKII levels were lower in the barrel cortexof T286A mutants than wild types. However, the effect of theT286A mutation appears to depend on the inability of ${alpha}$ CaMKIIto autophosphorylate rather than a reduction in ${alpha}$ CaMKII levels.In the visual cortex, the ${alpha}$ CaMKII^T286A mice show a 50% decreasein ${alpha}$ CaMKII (Taha et al., 2002). A decrease in total ${alpha}$ CaMKIIof 50% in the somatosensory cortex does cause a significantdecrease in cortical plasticity, as observed in the heterozygous ${alpha}$ CaMKII knock-out mice (Glazewski et al., 1996). However, theinhibition of plasticity in the T286A point mutant, which hasa 25% reduction in ${alpha}$ CaMKII, is far more severe than that ofthe ${alpha}$ CaMKII heterozygote, which has a larger reduction in ${alpha}$ CaMKII.Therefore, the greater effect on plasticity in the point mutant must be attributable to the dependence of plasticity on autophosphorylationat the T286 site.
Barrel cortex LTP
The results presented here show for the first time that neocorticalLTP is dependent on autophosphorylation of ${alpha}$ CaMKII. Regardlessof whether LTP is induced by theta-burst stimulation, pairingpresynaptic and postsynaptic depolarization, by sustained depolarization,or by spike pairing, LTP is absent in ${alpha}$ CaMKII^T286A mice. Thefact that the same conclusion is reached regardless of theLTP induction protocol used increases confidence that ${alpha}$ CaMKIIautophosphorylation is a basic requirement for induction ofLTP in the neocortex rather than a permissive or marginal factor. The fact that low-frequency pairing of presynaptic activitywith forced postsynaptic depolarization fails to induce LTPin the mutants shows that the mutation does not affect LTPby altering the transmission properties of the circuit.
Previous studies using knock-out mice had concluded that ${alpha}$ CaMKIIis required for hippocampal LTP (Silva et al., 1992). Thesame point mutation in ${alpha}$ CaMKII studied here has also been shownto almost completely block LTP in the Schaeffer collateral–CA1pathway of the hippocampus (Giese et al., 1998), where theresidual potentiation is attributed to an NMDA-independent component. However, LTP at the perforant path-dentate gyrus pathway showsno requirement for ${alpha}$ CaMKII autophosphorylation (Errington etal., 2002). The diversity of synaptic plasticity mechanismswithin the hippocampus and across other brain regions arguesagainst assuming that plasticity mechanisms discovered in CA1will necessarily be used in other cortical areas. However, our results suggest that the plasticity exhibited in the layerIV to II/III pathway of the cortex has relatively similar propertiesto that of CA1, as suggested previously (Kirkwood et al., 1993).
We studied the effects of spike-pairing as a more natural formof LTP induction that is likely to contribute to endogenousplasticity in the cortex (Feldman, 2000). Action potentialsare likely to back-propagate in the relatively short apical dendrites of mouse layer II/III pyramidal cells (Golding etal., 2002), are naturally evoked by sensory stimuli (Larkumand Zhu, 2002), are also known to affect spine calcium levelsin a nonlinear manner (Koester and Sakmann, 1998; Schilleret al., 1998), and clearly affect the scale and direction ofplasticity contingent on the timing of presynaptic and postsynapticactivity (Markram et al., 1997; Feldman, 2000). We confirmed that pairing the postsynaptic spike, so as to occur 10 msecafter the presynaptic spike, does produce LTP in neurons ofwild-type mice but not in ${alpha}$ CaMKII^T286A mutants.
Not all cells in the cortex showed LTP, although all slicesfrom wild types showed potentiation in the extracellular fields.This suggests some heterogeneity of cell type or pathway inthe barrel cortex. Glazewski and Fox (1996) previously notedthat whisker deprivation only causes a shift in the receptivefields of $~$ 50% of the cells recorded, which supports this view.However, when the response of a population of layer II/IIIcells is studied, whether by electrical stimulation of layerIV and extracellular recording in a slice or by whisker stimulation and extracellular recording of the evoked SEPs in the entireanimal, the subpopulation of cells that does potentiate tendsto dominate the response. Consequently, population recordingsreveal potentiation in every animal.
Cortical SEPs
The results presented here show for the first time that sensoryevoked synaptic responses are potentiated after single-whisker experience,and that this property of the barrel cortex is blocked in ${alpha}$ CaMKII^T286A mice. The field potentials evoked by whisker stimulation willreflect population activity over a limited distance in thecortex. The most influential factor contributing to the low-frequencycomponent of the field is the synaptic potentials. Therefore,a lack of potentiation in the ${alpha}$ CaMKII^T286A mice indicates aloss of sensory-evoked synaptic plasticity.
The synaptic potentials tend to occur synchronously in the barrelcortex, because whisker stimulation can be made with rapidonset (1 msec) and at a discrete moment in time, producinga high level of temporal summation. The small dipoles createdby the layer II/III pyramidal cells also summate spatiallyto some degree, although not as much as in the hippocampus,where the somata are more closely aligned. Both factors ensurea relatively large SEP and strong sinks and sources in theCSD analysis. Somatic and even dendritic action potentialscontribute relatively little to the CSD analysis, because theyare rapid events that tend not to summate temporally among cells. Whereas SEPs tend to measure several millivolts in amplitudeand last tens of milliseconds, spikes are rarely >2–300µV and last 1 msec. Spikes therefore compose <10%of the voltage at a very brief time point. In addition, spikesare sharply attenuated with distance far more than the lower-frequencycomponents. Finally, any local spikes are filtered out electronicallybefore additional analysis. Consequently, potentiation of the SEPs seen as a result of whisker deprivation is most likelya good reflection of the degree of potentiation of the excitatorysynaptic potentials within the cortex.
Toward a complete theory of experience-dependent plasticity
The weight of evidence is that experience-dependent plasticityis expressed in the cortex rather than subcortically (Fox, 1994, 2002; Glazewski and Fox, 1996; Wallace et al., 2001). Plasticity may be induced by whisker deprivation setting upa spike-firing pattern in the somatosensory system that inducessynaptic plasticity in a particular cortical pathway. Thosesynaptic plasticity mechanisms then require autophosphorylationof CaMKII. The activity patterns set up by whisker deprivationhave been studied recently by Kelly et al. (1999), who showedthat removing whiskers surrounding a particular spared whiskerleads to an increased firing in the barrel of the spared whiskerduring natural whisking behavior. The response to single-whiskerstimulation is unaffected by this manipulation, but the excitationproduced by a single whisker would normally be damped downby lateral inhibition generated by coincident activation ofthe surround whiskers during whisking. Presumably, a prolongedperiod of increased firing in the barrel of the spared whiskercauses potentiation in the postsynaptic targets of those layerIV cells (Fox, 2000), either by a spike-pairing mechanism(Feldman, 2000) or simply because of the increased firing rate.
We have shown that a variety of firing patterns do lead to synaptic plasticity in the barrel cortex, either spike pairing or theta-burstfiring. Theta-burst frequencies are similar to those generatedduring whisking behavior in the rodent and might be expectedto occur with higher-frequency bursts in single-whisker micethan in normal mice. Although synaptic plasticity can occurin the absence of postsynaptic spikes, in vivo it is very likelythat postsynaptic spikes will occur during sensory responses,which makes induction of plasticity by spike pairing highly relevant.
The results of this study show that potentiation is dependenton ${alpha}$ CaMKII autophosphorylation. Why autophosphorylation is importantfor potentiation is not entirely clear. Evidence suggests itis not necessary for expression of LTP (Lisman et al., 2002),although it is required for induction. Nevertheless, autophosphorylationdoes last for $~$ 1 hr after induction of LTP in the hippocampusand would be expected to prolong the capacity of the kinaseto phosphorylate and enable it to translocate to the postsynapticdensity (Shen and Meyer, 1999). Both factors would tend toimprove the chances of ${alpha}$ CaMKII phosphorylating synaptic substratesincluding AMPA receptors at the serine 831 site of the glutamatereceptor type 1 (GluR1) subunit, a process known to increase conductance and therefore produce potentiation (Barria et al.,1997). The fact that LTP is not entirely abolished in micelacking the GluR1 subunit (Hoffman et al., 2002) implies thatat least one other mechanism is involved.
The results of this and other studies in the barrel cortex offera possibility of a complete description of a plasticity processfrom circuit behavior through to molecular mechanism. Thisstudy makes a connection between the neuronal circuit behaviorand synaptic plasticity by showing that both experience-dependentplasticity and LTP critically depend on ${alpha}$ CaMKII autophosphorylationin the same pathway.

   Footnotes

Received Jan. 24, 2003; revised Mar. 5, 2003; accepted Mar. 7, 2003.
This work was supported by Medical Research Council Grant G99009 [GenBank] 31to K.F. We thank Phil Blanning for genotyping and John Curryfor help with the histology.
Correspondence should be addressed to Prof. Kevin Fox, Schoolof Biosciences, Cardiff University, Museum Avenue, CardiffCF10 3US, UK. E-mail: foxkd{at}cf.ac.uk.
S. Glazewski's present address: McKay Institute of Communicationand Neuroscience, Keele University, Staffordshire ST5 5BG,UK.
P. Pakhotin's present address: School of Biological Sciences,Manchester University, Manchester M13 9PT, UK.
Copyright © 2003 Society for Neuroscience 0270-6474/03/234428-09$15.00/0
^* N.H., S.G., and P.P. contributed equally to this work.

   References

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Materials and Methods
Results
Discussion
References

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