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The Journal of Neuroscience, July 1, 2002, 22(13):5719-5726
Transgenic Calmodulin-Dependent Protein Kinase II Activation: Dose-Dependent Effects on Synaptic Plasticity, Learning, and Memory
Rafael Bejar1, Rie Yasuda2, 4, Harmen Krugers3, Kristin Hood1, and Mark Mayford1, 4 1 Neurosciences Graduate Program, University of California at San Diego, La Jolla, California 92093, 2 Genomics Institute of the Novartis Research Foundation, San Diego, California 92121, 3 Swammerdam Institute for Life Sciences, Section of Neurobiology, University of Amsterdam, 1090GB The Netherlands, and 4 Department of Cell Biology, The Scripps Research Institute, La Jolla, California 92037
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Genetic disruption of calmodulin-dependent protein kinase II (CaMKII) function alters hippocampal synaptic plasticity and memory in mice. We used transgenic mice carrying a tetracycline-regulated, calcium-independent form of CaMKII (CaMKII-Asp286) to investigate the role of CaMKII activation on synaptic plasticity and behavior. Mice expressing low levels of a CaMKII-Asp286 transgene have facilitated low-frequency (5 Hz)-induced long-term potentiation (LTP), whereas mice with high levels of transgene expression have a deficit in this form of plasticity. Behavioral impairments on fear-conditioned memory and visible water maze correlate with the level of CaMKII-Asp286 expression. Mice with high levels of CaMKII-Asp286 have reversible, compensatory changes in the expression of genes associated with inhibitory neurotransmission. These results demonstrate that in the hippocampus, CaMKII activation facilitates the induction of low-frequency LTP, but at high levels of expression, compensatory mechanisms act to inhibit the induction of this form of LTP. The most severe behavioral impairments are associated with activation of this compensatory mechanism.
Key words: memory; CaMKII; mice; transgenic; tetracycline; genetic compensation; long-term potentiation
INTRODUCTION
In the CA1 region of the hippocampus, both biochemical and pharmacological studies demonstrate that activation of calmodulin-dependent protein kinase II (CaMKII) is required for the establishment of long-term potentiation (LTP) (Malenka et al., 1989
; Malinow et al., 1989
gene results in mice with deficient hippocampal LTP and spatial-memory impairments (Silva et al., 1992a
Complementary studies in transgenic mice expressing a constitutively active calcium-independent mutant form of CaMKII failed to support the view that CaMKII activation alone is sufficient to produce LTP (Bach et al., 1995
Although genetically modified mice are a powerful tool for the specific molecular manipulation of a whole-animal model, there are two difficulties in interpreting results of such experiments in terms of the function of the gene under study (Mayford and Kandel, 1999
MATERIALS AND METHODS
CaMKII-Asp286 transgenic mice. Transgenic mice carrying a Ca2+-independent CaMKII transgene (CaMKII-Asp286) under the control of the tetracycline transactivator (tTA) were generated as described previously (Mayford et al., 1996
Northern blots. Immediately after killing, the mouse brain was removed and immersed in ice-cold PBS. The appropriate brain region was dissected, and total RNA was isolated using Trizol reagent (Sigma, St. Louis, MO) as recommended by the manufacturer. RNA was separated by electrophoresis on a formaldehyde-containing agarose gel, blotted to a nylon membrane, and hybridized at 55°C overnight with PerferctHyb (Sigma) containing 106 cpm of a radiolabeled DNA probe per milliliter of hybridization solution. The labeled blot was washed with 0.2× SSC and 0.1% SDS, and the hybridization signal was quantified using a phosphorimager.
Reverse transcription-PCR detection of CaMKII-D286 transgene mRNA. Reverse transcription (RT) was performed with the PerkinElmer Life Sciences (Emeryville, CA) rtTH I polymerase RNA PCR kit according to the manufacturer's instructions. The complimentary oligonucleotide used for RT of CaMKII RNA was 5'-CTCTGGTTCAAAGGCTGTCA-3'. After the RT step, the second PCR oligonucleotide was added: 5'-AGATGCTGACCATCAACCCA-3'. Samples were cycled 40 times through the following amplification series: 30 sec at 94°C, 30 sec at 55°C, and 60 sec at 72°C. This protocol produces a 401 bp product from both native and transgenic CaMKII mRNA.
Equal amounts of RT-PCR product (as determined by gel band intensity) were either run on a 1.7% gel and blotted onto a nylon membrane by capillary transfer with 0.4 M NaOH or vacuum applied to a nylon membrane. To detect the CaMKII-Asp286 transgene, blots were hybridized overnight at 37°C with a 32P-labeled oligonucleotide specific to the Asp286 mutation (5'-CTTCAGGCAGTCGACGTCCTCCTGTCTGTG- 3'). The hybridization solution contained 50% formamide, 100 mg/ml dextran sulfate, 25 mM HEPES, pH 7.5, 1 mM EDTA, 0.1 mg/ml denatured salmon sperm DNA, 0.2 mg/ml poly-rA, 5× Denhardt's reagent, 600 mM NaCl, and 0.1% SDS. After washing in 0.2× SSC, the blot was exposed to film and quantified using a phosphorimager. Loading controls were performed by probing the original blot, or a replica blot, with an oligoprobe complementary to wild-type CaMKII (5'-CTTCAGGCAGTCCACGGTCTCCTGTCT-3').
Visible water maze. The water-maze apparatus consisted of a 1.2-m-diameter water-filled pool. In the pool, there was a 10-cm-diameter circular platform that lay flush with the surface of the water. Before training, animals were handled in the testing room for 7 d. Training begins 1 d after the final day of handling. Mice were individually placed onto the raised platform, to which a visible flag had been attached, and allowed to acclimate for 15 sec. Mice were then placed in the water and allowed to swim for 15 sec, after which time they were guided back to the platform to rest for another 15 sec. After acclimatization, mice were placed at a start position along the wall of the tank and given 60 sec to find the visibly flagged platform. If they did not find it in 60 sec, they were led back to the platform. Once on the platform, mice were given 30 sec to rest before being returned to their home cage. Two more visible-platform trials were conducted with the platform, and start locations varied in a pseudorandom manner. Additional days of training (without acclimatization) to a visible platform (three trials per day) may be given to some groups.
Fear-conditioning. Mice were trained in a Plexiglas enclosure containing a wire grid floor, an overhead speaker, and external lighting (Freeze Monitor; San Diego Instruments, San Diego, CA). After a 3 min baseline period, three 20-sec-long tones (77 dB, 2.8 kHz) were played with a 1 min intertrial interval. A 0.75 mA foot shock was delivered during the last 1.5 sec of each tone. Twenty-four hours after training, mice were again placed in the original training enclosure for 3 min, and freezing was assessed either by visual scoring or by computer analysis of video frame capture. Two hours later, mice were placed in a new enclosure. After a 3 min baseline exposure, a series of three tones identical to that given in the training session was played, and freezing was scored during the tones.
Field potential electrophysiology. Transverse slices (400 µm thick) of mouse hippocampus were prepared and maintained in an interface slice chamber while being perfused with artificial CSF (aCSF) at 29-31°C. The aCSF contained the following (in mM): 124 NaCl, 4.4 KCl, 25 NaHCO3, 1.2 Na2HPO4, 1.2 MgSO4, 10 glucose, and 2 CaCl2. For baseline recording, EPSPs were elicited once every 50 sec (0.02 Hz) using nichrome wire bipolar stimulation electrodes (0.01 msec pulse duration) placed in the stratum radiatum of the CA1 region. The resulting potential was monitored using low-resistance glass microelectrodes (5-15 M
, filled with aCSF) also placed in the stratum radiatum of CA1. In each experiment, the maximal field EPSP amplitude was first determined by gradually increasing the stimulation intensity until the EPSP amplitude reached a saturating level. The stimulation intensity was subsequently decreased so as to evoke a response that was ~50% of the maximal EPSP amplitude. In all experiments, baseline synaptic transmission was monitored for 20 min before low-frequency stimulation was delivered. Slices were stimulated at 5 Hz for 30 sec (150 pulses), and synaptic responses were then monitored at 0.02 Hz for 1 additional hour.
Gene expression analysis. Gene chip experiments were performed essentially as described previously (Sandberg et al., 2000
Samples were obtained from mice expressing high levels of CaMKII-Asp286 (two B13-DEV mice and one B13 mouse) and from CaMKII-Asp286 mice expressing lower levels of their transgene (one B13-DEV mouse and two B13 mice). Two wild-type littermates were included as controls. For the expression of a gene to be considered changed, its level had to be scored as higher or lower in at least four of the six possible comparisons and had to have changed more than twofold.
RESULTS
Suppression and induction of a tTA-controlled CaMKII-Asp286 transgene
The mice used in this study carry a mutant Ca2+-independent CaMKII transgene, CaMKII-Asp286, under the control of a tetracycline-responsive promoter (Gossen and Bujard, 1992
To suppress gene expression during gestation and still allow for rapid induction in the adult, we delivered the tetracycline analog Dox in food at a dose of 40 mg/kg mouse chow. After Dox withdrawal, the transgene was rapidly activated in neurons throughout the forebrain (Fig. 1A), with maximal expression reached at 2 weeks after Dox withdrawal (Glazewski et al., 2001
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Figure 1. Transgene regulation. A, Expression of transgenic CaMKII-Asp286 mRNA is shown by in situ hybridization in these half-coronal forebrain sections taken from B13-DEV(high) mice. Mice treated with a low-dose doxycycline diet for >3 weeks show no expression (On DOX). Transgene mRNA expression is readily apparent within 2 d and is present at high levels at 14 d after mice are switched to a Dox-free diet. Brain slices used in this figure were prepared in parallel, probed with the same radiolabeled oligonucleotide, and exposed to film for the same amount of time. B, Mice raised with their transgene suppressed (B13) do not express as much CaMKII-Asp286 mRNA as adults compared with mice that have expressed the transgene throughout development (B13-DEV). The average level of expression in B13-DEV mice has been normalized to 100%. For hippocampal expression, p < 0.03; for striatal expression, p < 0.001.
Correlation between behavioral deficits and CaMKII-Asp286 expression levels
Figure 2A shows a schematic representation of the transgene expression history and behavioral testing points in our first experiment. Animals were allowed to develop with the transgene either on or off. Transgene expression was subsequently suppressed with Dox in both groups and reactivated before behavioral testing. This produced two groups of mice that differed in level of transgene expression at testing as well as in their developmental exposure to the transgene. We will refer to these groups as B13-DEV(high) and B13(low) to indicate both developmental exposure and level of transgene expression at testing.
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Figure 2. Behavioral effects of CaMKII-Asp286 transgene expression. A, Timeline showing regulation of the CaMKII-Asp286 transgene. B13 mice (gray line) had their transgene off throughout development. In B13-DEV mice (black line), the transgene was expressed during development and was first suppressed at 6 weeks of age. At ~11 weeks of age, both groups of mice had their transgene induced for 21 d before behavioral testing. B, The latency for mice to reach the visible platform is shown as a function of training trial. Across all trials, B13-DEV(high) mice have longer latencies than B13(low) mice (p < 0.02), which have longer latencies than control mice (p < 0.001). C, Degree of freezing in response to training, context, and auditory cues after tone-shock pairings. Despite having similar degrees of baseline freezing (p > 0.05 by ANOVA), B13-DEV(high) mice freeze less to context and cues than do B13(low) mice (p < 0.015) and control mice (p < 0.001).
Animals were first tested in the visible-platform version of the water maze. As shown in Figure 2B, the two transgenic groups differed from wild-type controls as well as from each other, with the B13-DEV(high) animals being the most severely impaired. A two-way ANOVA with repeated measures showed a significant main effect of group (F(2,36) = 26.9; p < 0.001) and trial (F(5,180) = 8.67; p < 0.001), and a post hoc Scheffé test showed that the two transgenic groups differed from each other (p < 0.02) and from the wild-type controls (p < 0.001). Thus, both groups of mice were impaired on this simple hippocampus-independent task. The impairment on the initial training trial suggests that some sensory, motor, or motivational impairment is responsible for the deficit in these mice. The striatum has been implicated in this simple form of learning, and it is likely that expression of the transgene in this structure contributes to this deficit (Devan et al., 1996
We subsequently tested performance of the two groups in a simple fear-conditioning task. Again, the mice showed the same general pattern of deficits, with the animals expressing high levels of the transgene showing a more severe impairment (Fig. 2C). A two-way ANOVA showed a significant effect of group (F(2,35) = 14.9; p < 0.001) but not of test (cued or context), and a post hoc Scheffé test showed that the B13-Dev(high) group differed significantly from both the wild-type control group and the B13(low) group [B13-DEV(high) vs control, p < 0.001; B13-DEV(high) vs B13(low), p < 0.02].
The interpretation of these results is complicated by the fact that the two transgenic groups differed not only in the level of transgene expression during behavioral testing but also in exposure to the transgene during development. To distinguish between dose effects and developmental effects, we isolated mRNA from each of the animals that had undergone behavioral testing and determined the level of transgene expression. Figure 3 shows the correlation between levels of transgene expression in individual animals and their performance on the two different behavioral tests. Although the two groups differed on average in transgene expression level (Fig. 1B), there was significant overlap of individual values. The correlation between the level of transgene expression in individual animals and the severity of the behavioral deficit was highly significant.
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Figure 3. Correlations between CaMKII-Asp286 gene dose and behavioral performance. A, Contextual fear-conditioned freezing 24 hr after training is plotted as a function of CaMKII-Asp286 mRNA levels in the hippocampus. The R2 value for all transgenic mice is 0.683 (p < 0.001). B, The average latency for mice to reach the visible water-maze platform on day 2 of training is plotted as a function of hippocampal CaMKII-Asp286 mRNA levels. The R2 value for all transgenic mice is 0.527 (p < 0.001). Regardless of transgene exposure during development, animals with a greater transgene dose as adults were more likely to have severe deficits on these tasks. One unit of expression is defined as the amount of mRNA expressed by mice carrying only the tetO-linked CaMKII-Asp286 transgene (no tTA transgene). The control group includes six wild-type mice and three mice carrying only the tetO-linked CaMKII-Asp286 transgene.
Behavioral deficits are reversible with transgene suppression
We subsequently examined the reversibility of the behavioral deficits produced in the B13-Dev(high) group of animals. Figure 4A shows the regulation of transgene expression and the timing of behavioral testing. Animals trained and tested with the transgene on showed a severe impairment in contextual fear conditioning (Fig. 4B). After suppression of the transgene, the memory was still significantly impaired, indicating that transgene expression disrupted the encoding of the memory rather than merely affecting performance of the freezing response. Retraining of animals with the transgene suppressed resulted in the formation of wild-type levels of conditioned fear. This demonstrates that although the animals expressed high levels of the transgene during development, the impairment on this task could not be a result of any permanent developmental abnormality. Finally, re-expression of the transgene severely disrupted the freezing of animals conditioned with the transgene suppressed. Similar results were seen in the visible-platform water maze task. As shown in Figure 4C, animals trained with the transgene on were strongly impaired at finding the visible platform in the water maze. When the transgene was suppressed, animals rapidly acquired the task to wild-type levels of performance.
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Figure 4. Reversible behavioral deficits in B13-DEV(high) mice. A, Timeline showing the CaMKII-Asp286 transgene activation pattern for the experiment shown in B. B, Contextual freezing is impaired in B13-DEV(high) mice 24 hr after training with the transgene on and at 6 weeks after transgene suppression (measured during the baseline period immediately before retraining). Twenty-four hours after retraining with the transgene off, B13-DEV(high) mice show normal freezing to context compared with controls. When the transgene is induced after normal learning, B13-DEV(high) mice have a complete lack of freezing to the context learned previously. **p < 0.001. C, B13-DEV(high) mice fail to locate a visible platform in the water maze, whereas controls acquire this task readily. After transgene suppression, B13-DEV(high) mice learn to locate the visible platform (performance on last two trials, wild-type vs B13 mice; p = 0.14; NS).
Low levels of CaMKII facilitate 5 Hz LTP induction, but high levels impair 5 Hz LTP induction
We have previously shown a deficit in Schaffer-collateral LTP induced by low-frequency stimulation in several lines of CaMKII-Asp286 transgenic mice, including the B13 mice used in the present study (Mayford et al., 1995
The most striking finding from this experiment (Fig. 5) was that transgenic mice expressing low levels of the CaMKII-Asp286 transgene did not show a shift toward LTD, as had been reported previously, but instead showed an enhanced level of LTP after 5 Hz stimulation (F(1,28) = 6.23; p < 0.05). Consistent with our previous study, the mice expressing high levels of the transgene had an impairment in LTP induced by the 5 Hz stimulation protocol (F(1,28) = 4.26; p < 0.05). Unlike the behavioral results, which demonstrate a quantitative difference in the severity of deficits between the two groups of mice, these LTP results suggest that there is a threshold dose of constitutive CaMKII activity at which there is a qualitative switch from enhanced 5 Hz LTP to impaired 5 Hz LTP.
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Figure 5. CaMKII-Asp286 expression alters theta-frequency LTP. Hippocampal LTP induced by 5 Hz stimulation in B13(low) and B13-DEV(high) groups during CaMKII-Asp286 expression is shown. Hippocampal slices from B13(low) and B13-DEV(high) groups were stimulated at 0.02 Hz while EPSPs were recorded from CA1 dendritic fields. After 20 min of baseline, slices were stimulated at 5 Hz for 30 sec, followed by 1 hr of 0.02 Hz recording. Note how B13(low) and B13-DEV(high) mutants have opposing responses to 5 Hz stimulation. B13-DEV(high) mutants have an LTP deficit, whereas B13(low) mutants trend toward enhanced LTP at this stimulation frequency. Representative EPSPs for each group of animals tested are shown before and after the 5 Hz stimulation. Calibration, 10 msec, 2 mV.
Compensatory changes in gene expression at high levels of CaMKII-Asp286
Calmodulin-dependent protein kinases have been shown to modulate gene expression (Enslen and Soderling, 1994
To determine whether mRNA levels of GAD65 and Tac were affected in the CaMKII-Asp286 mice presented here, we performed Northern blots on striatal mRNA obtained from the B13-DEV(high) and B13(low) mutant mice described in Figure 2. Expression of these genes was elevated in the transgenic mice and was significantly correlated with levels of striatal CaMKII-Asp286 mRNA (Fig. 6A,B). The results of an additional Northern blot demonstrate that the increased levels of both GAD65 and Tac are reversible with transgene suppression (Fig. 6C). The reversible nature of this change parallels that of the behavioral phenotype in B13-DEV(high) mice.
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Figure 6. Striatal GAD65 and tachykinin expression correlates with CaMKII-Asp286 expression. A, Striatal expression of CaMKII-Asp286 and GAD65 co-vary, with an R2 value for all transgenic mice of 0.722 (p < 0.001). B, Striatal expression of CaMKII-Asp286 and Tac co-vary, with an R2 value for all transgenic mice of 0.865 (p < 0.001). Expression levels were assayed by Northern blot of total striatal RNA and normalized for levels of tubulin mRNA. One unit of expression is defined as the amount of mRNA expressed by mice carrying only the tetO-linked CaMKII-Asp286 transgene (no tTA transgene). The control group includes four wild-type mice and two mice carrying only the tetO-linked CaMKII-Asp286 transgene. C, Northern blots for GAD65 and Tac mRNA. Whole-forebrain RNA from B13-DEV(high) mutant mice with their transgene induced (High ON) and suppressed (High OFF) as well as from B13(low) mutants with their transgene induced (Low ON) is probed for GAD65. At this exposure, significant expression is seen only in the B13-DEV(high) mice tested with their transgene expressed (High ON).
These results suggest that in addition to the role of the CaMKII-Asp286 transgene itself, compensatory changes in gene expression may underlie the behavioral phenotypes observed in these animals. We examined gene expression changes in the hippocampus from animals expressing either high or low levels of the CaMKII-Asp286 transgene. We used the mouse U74 GeneChip for these comparisons (Tables 1 and 2). The transcriptional responses in the two groups were qualitatively different. Only two genes showed expression changes in both the high- and low-expressing groups and could therefore be directly linked to the levels of CaMKII-Asp286 transgene expression (spi2, B-cell-specific protein). Many of the genes that are upregulated specifically in the hippocampus of animals expressing high levels of CaMKII-Asp286 are also known to be upregulated in response to synaptic activity and LTP-inducing stimuli [transforming growth factor-
-inducible early growth response, zif/268, Jun-B, pip92, neuropeptide Y (NPY), inhibin
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Table 1. Changes in hippocampal gene expression between mice expressing high levels of CaMKII-Asp286
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Table 2. Changes in hippocampal gene expression between mice expressing low levels of CaMKII-Asp286
DISCUSSION
Genetically modified mice have been used extensively to address the molecular mechanisms of complex neurobiological phenomena such as synaptic plasticity, learning, and memory. One of the difficulties of this approach is dissociating primary effects on learning mechanisms from potential secondary effects that a genetic modification may have on neuronal development or on compensatory changes in the expression of other genes (Mayford and Kandel, 1999
Using the Tet system, we have shown that transgene expression can be effectively suppressed during development with low levels of Dox that allow relatively rapid transgene induction in adult animals. A surprising finding was that suppression of transgene expression during development led to a reduction in the adult levels of gene expression that could be obtained. Although this could result from residual Dox in those animals that were exposed to the drug during gestation, we think it is more likely a result of alterations in genomic DNA in the neighborhood of the tetO-linked transgene. We favor this view because even prolonged withdrawal from Dox does not lead to consistently high levels of expression in these mice, and in a second line of tetO-linked CaMKII-Asp286 transgenic mice, we found that developmental suppression of transgene expression completely eliminated the ability to induce the transgene in adult animals (Hood, unpublished results). This may result from changes in chromatin structure or DNA methylation at the inactive transgene locus (Pikaart et al., 1998
Previous studies using pharmacological inhibitors and knock-out mice support the view that CaMKII activation and autophosphorylation at Thr286 is required for the induction of LTP (Malenka et al., 1989
Together, these results suggest that the primary effect of CaMKII-Asp286 expression is to facilitate the induction of LTP, but that at high levels of expression, compensatory changes mask that effect. This is consistent with the view that CaMKII activation is necessary for LTP induction. Lisman and Zhabotinsky (2001)
Activation of CaMKII to low levels produces deficits in visible-platform water maze performance only in adult animals. This is not a hippocampus-dependent task and is most likely mediated by physiological effects in other brain regions, such as the striatum (Devan et al., 1999
These results are consistent with the idea that the primary effect of CaMKII activation is excitatory, possibly by facilitating the induction of LTP. The shift in LTP threshold at low levels of transgene expression results in mild behavioral impairments that may be attributable to inappropriate synaptic weight changes in response to a given environmental stimulus. At high levels of transgene expression, compensatory upregulation of inhibitory neurotransmitter systems acts to oppose increased excitation and prevent excessive neuronal activity and seizure, at least in the hippocampus. In the striatum, in which the medium spiny neurons are GABAergic projection neurons, the changes in gene expression may represent an increase in striatal output resulting from facilitated corticostriatal transmission (Hood, unpublished results). The severe behavioral impairments could result from these secondary changes in transmission.
How do these results reflect the role of CaMKII activation in response to natural stimuli? Behaviorally induced changes in CaMKII activity have not been studied extensively; however, after LTP induction, autophosphorylated CaMKII is elevated for at least 1 hr (Fukunaga et al., 1993
These results highlight some of the difficulties in studying genetically modified mice in general and in a highly adaptive system such as the brain in particular. The introduction of a single genetic alteration, even in an inducible manner, can have significant downstream consequences that can complicate interpretation. The advent of GeneChip technology coupled with the sequencing of the mouse genome should make it theoretically possible to detect many of the compensatory changes in gene expression, reflected at the RNA level, that occur in a given mutant animal. This level of analysis, coupled with regulated genetic systems such as Tet and more anatomically restricted promoters, should enhance our ability to understand how single gene changes exert their effects on complex neurobiological processes.
FOOTNOTES Received Jan. 21, 2002; revised April 12, 2002; accepted April 12, 2002.
This work was supported by grants from the National Institutes of Health (M.M., R.B.), the McKnight Foundation (M.M.), and the Klingenstein Foundation (M.M.).
Correspondence should be addressed to Mark Mayford, Cell Biology, ICND202, The Scripps Research Institute, La Jolla, CA 92037. E-mail: mmayford{at}scripps.edu.
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