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Previous Article | Next Article
The Journal of Neuroscience, November 1, 1999, 19(21):9538-9549
Regulation of Learning by EphA Receptors: a Protein Targeting Study
R. Gerlai1, N. Shinsky1, A. Shih1, P. Williams2, J. Winer2, M. Armanini1, B. Cairns3, J. Winslow1, W.-Q. Gao1, and H. S. Phillips1 Genentech,
Inc., Departments of 1 Neuroscience, 2 Research BioAssay, and 3 Pathology, South San Francisco, California 94080
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EphA family receptor tyrosine kinases and their ephrin-A ligands are involved in patterning axonal connections during brain development, but until now a role for these molecules in the mature brain had not been elucidated. Here, we show that both the EphA5 receptor and its ephrin-A ligands (2 and 5) are expressed in the adult mouse hippocampus, and the EphA5 protein is present in a phosphorylated form. Because there are no pharmacological agents available for EphA receptors, we designed recombinant immunoadhesins that specifically bind to the receptor binding site of the ephrin-A ligand (antagonist) or the ligand binding site of the EphA receptor (agonist) and thus target EphA function. We demonstrate that intrahippocampal infusion of an EphA antagonist immunoadhesin leads to impaired performance in two behavioral paradigms, T-maze spontaneous alternation and context-dependent fear conditioning, sensitive to hippocampal function, whereas activation of EphA by infusion of an agonist immunoadhesin results in enhanced performance on these tasks. Because the two behavioral tasks have different motivational, perceptual, and motor requirements, we infer the changes were not caused by these performance factors but rather to cognitive alterations. We also find bidirectional changes in gene expression and in electrophysiological measures of synaptic efficacy that correlate with the behavioral results. Thus, EphA receptors and their ligands are implicated as mediators of plasticity in the adult mammalian brain.
Key words: EphA tyrosine kinase receptor; immunoadhesin; learning; mouse; hippocampus; inbred strain; LTP
INTRODUCTION
EphA receptors represent the largest subfamily of receptor tyrosine kinases (Friedman and O'Leary, 1996
). The ephrin-A ligands interact with EphA receptors to mediate repulsive axonal guidance in patterning the developing nervous system (Drescher et al., 1995
EphA receptors were shown to play a role in determining patterns of synapse formation in development (Drescher et al., 1995
To target EphA5 function, we use a novel strategy termed protein targeting (Gerlai et al., 1998b
In the present paper, we focus on the analysis of behavioral changes elicited by intrahippocampal infusion of the EphA antagonist and agonist immunoadhesins and also study potential underlying mechanisms, including gene expression changes and synaptic plasticity. We demonstrate, for the first time, that EphA receptors play a significant role in the adult brain in which they influence cognitive function.
MATERIALS AND METHODS
Animals and housing. Experimental mice (males) from inbred strains C57BL/6 and DBA/2 were 3-4 months old and were housed in groups of 10 under standard conditions described previously (Gerlai et al., 1998b
In situ hybridization. For EphA5 in situ hybridization, 4-month-old DBA/2 and C57BL/6 mouse brains were fresh frozen with powdered dry ice. Sections were processed by a method described previously (Melton et al., 1984
RT-PCR. Total RNA was isolated using the Qiagen (Hilden, Germany) RNeasy Mini Kit from 50 mg mouse hippocampi freshly frozen in liquid nitrogen. RNA was aliquoted and stored at
70°C until used. Oligonucleotide probes and primers were designed to recognize the genes using the Primer Express software [Applied Biosystems (Foster City, CA) and Perkin-Elmer (Emeryville, CA)]. Real-time quantitative RT-PCR (TaqMan) was performed and analyzed using the Promega (Madison, WI) Access RT-PCR System in the ABI Model 7700 Sequence Detection system (Gibson et al., 1996
Western blot. The methods are described in detail previously (Winslow et al., 1995
Stereotaxic surgery and infusion. Using a stereotaxic frame, mice received bilateral intrahippocampal implantation of cannulas as described in detail previously (Gerlai et al., 1998b
Immunoadhesins. The design and production of immunoadhesins, as well as their advantages, including stability and detection, have been described and discussed in detail previously (Winslow et al., 1995
Immunohistochemistry. The methods followed standard protocols (Gerlai et al., 1998b
biotin-peroxidase complex (Elite ABC kit; Vector Laboratories, Burlingame, CA), rinsed, and developed using a standard diaminobenzidine reaction (Enhanced Metal; Pierce, Rockford, IL).
T-maze continuous spontaneous alternation task. The procedure followed the methods developed and described previously (Gerlai, 1998a
Fear conditioning. The methods have been described in detail previously (Gerlai, 1998b
Electrophysiology. Transverse 300 µm hippocampal slices were submerged in a recording chamber (Fine Science Tools Inc., Foster City, CA), continuously perfused with 30°C oxygenated (95% O2-5% CO2) ACSF for at least 1 hr before recording. A bipolar glass electrode filled with ACSF stimulated Schaffer collaterals. Field EPSPs (fEPSPs) elicited by single-pulse stimulation at 0.2 Hz were recorded in CA1 stratum radiatum by a glass electrode filled with ACSF. Input/output (I/O) characteristics and ratio of the fEPSP slope to the presynaptic fiber volley (PSFV) amplitude were used to estimate basal synaptic transmission. I/O characteristics, recorded by applying gradually increased (in 20 steps increments) stimulus intensity to evoke fEPSP from minimum to maximum slope, were estimated by Michaelis-Menten sigmoid curve fit. Km50 was taken as a 50% point between the threshold and maximal response (A/DVANCE software; McKellar Designs). Baseline was recorded for 1 hr with the stimulus intensity set to evoke a fEPSP that was 30-50% of the maximal slope. Paired-pulse facilitation (PPF) was evoked by applying paired pulses of the same intensity as for baseline recording with interpulse intervals of 50, 100, 150, 200, and 250 msec. LTP was elicited by applying four trains of 100 Hz tetanus (1 sec duration, 20 sec apart), with the same stimulus intensity as for the baseline and PPF. In our attempt to test the potential improving effects of ephrinA5-IgG on synaptic plasticity in slices from C57BL/6 mice, we used another protocol of tetanization that is subthreshold for LTP induction. In this set of experiments (for results, see Fig. 12), one train of 100 Hz tetanus was applied for 1 sec with stimulus intensity set to evoke a fEPSP 10-15% of maximal slope. Recordings in all experiments were made with an Axoprobe-1A amplifier (Axon Instruments, Foster City, CA) interfaced with a Power Macintosh 7100/66 computer (Apple Computers, Cupertino, CA). Data were acquired, digitized, and analyzed using A/DVANCE software (McKellar Designs).
Statistical analysis. Data were analyzed by t test, repeated-measures ANOVA, and post hoc Tukey's honestly significant difference (HSD) test. Variance homogeneity was tested by Bartlett's test. Only relevant main effects are presented; detailed data analysis results are available on request.
RESULTS
Expression pattern of EphA5 and its ligands in the adult mouse brain
Using in situ hybridization (Melton et al., 1984
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Figure 1. The EphA5 receptor and its ligands are expressed in the adult mouse hippocampus. In situ hybridization (coronal sections with antisense probe) for EphA5 mRNA expression in the brain of C57BL/6 (A-C) and DBA/2 (D-F) strains of mice. A section with sense (control) probe (H) is also shown. Approximate position of sections from bregma are (in mm): A, D, +0.75; B, E, H, CT). Sample sizes (n) indicate the number of mice analyzed. Note that larger values mean smaller original mRNA amount in the hippocampal tissue sample. Also note that amplification characteristics are unique to each gene; therefore, comparison from one gene to another is not valid. I, Western blot for phosphorylated EphA5. Each lane represents a hippocampal tissue sample from an individual mouse. Both DBA/2 (a1, a2) and C57BL/6 (b1, b2) strain of mice exhibit a prominent signal.
Infusion of immunoadhesins into the hippocampus
To confirm that the antagonist immunoadhesin EphA5-IgG and the agonist immunoadhesin ephrinA5-IgG binds to their relevant targets under conditions similar to those of the in vivo application we were planning (37°C; ALZET micro-osmotic pump), ELISA essay was performed. The immunoadhesin solution was injected into a micro-osmotic pump, the pump was placed in a thermostat at 37°C, and the solution was sampled over a 10 d period. The results (data not presented) showed that both immunoadhesins retained a significant and specific binding capacity.
To study EphA function, we infused the antagonist or agonist immunoadhesin bilaterally into the hippocampus using micro-osmotic pumps (Gerlai et al., 1998b
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Figure 2. Immunohistochemical staining for the IgG domain of the immunoadhesin reveals pronounced hippocampal diffusion of the protein after 7 d intrahippocampal infusion from micro-osmotic pump. The right hemisphere with EphA5-IgG infusion in C57BL/6 mice is shown: A, anterior (bregma
Consistent with its antagonist action, EphA5-IgG was shown previously to impair phosphorylation of the EphA5 receptor (Winslow et al., 1995
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Figure 3. EphA5 receptor phosphorylation is induced by in vivo infusion of the agonist ephrinA5-IgG in hippocampal tissue samples. After immunoprecipitation with anti-EphA5 antibody, phosphorylation levels were detected by anti-phosphotyrosine kinase antibody. Each lane represents hippocampal tissue from an individual mouse: a, ephrinA5-IgG infusion; b, CD4-IgG infusion. Lanes 1-4 represent samples from C57BL/6; lanes 5-8 represent samples from DBA/2. The monomer (EphA5) protein is indicated.
To determine whether EphA receptors mediate neural function, we focussed our attention to the hippocampus because of the expression pattern of EphA5 and also because of the availability of behavioral paradigms and electrophysiological methods sensitive to detect dysfunction of this structure. We put considerable emphasis on behavioral analysis because it offers a sensitive way to detect neural functional changes (Gerlai, 1996c
Behavioral changes elicited by immunoadhesin infusion
We use the availability of two inbred strains of mice, C57BL/6 and DBA/2, that exhibit striking differences in hippocampal function at the behavioral level (Paylor et al., 1994
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Figure 4. EphA5-IgG infusion impairs T-maze continuous alternation in C57BL/6 mice in a 15 trial alternation session. EphA5-IgG infusion, hatched bar, n = 23; CD4-IgG infusion, black bar, n = 22. One choice was allowed at each trial. Alternation rate is a ratio between the alternating choices and total number of choices. A, Significant difference was found in alternation rate (t = 3.528; df = 43; p < 0.001). B, No significant difference was found between groups in time spent to complete the 15 choices (t = 0.915; df = 43; p > 0.36). Error bars represent SEM.
The deficit in EphA5-IgG-infused mice was further characterized using context-dependent fear conditioning (CDFC), a configural learning task also found sensitive to hippocampal dysfunction (Kim and Fanselow, 1992
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Figure 5. EphA5-IgG infusion impairs learning performance in a context-specific manner in fear conditioning in C57BL/6 mice. In the CDFC paradigm, mice associate two substantially different types of cues with a negative reinforcer, an electric foot shock. The shock is paired with a simple associative cue, a tone, in a shock chamber characterized by multiple contextual cues. A, During training, mice were given three 20 sec tone signals (solid horizontal bars) that coterminated with 1-sec-long electric shocks (0.5 mA; arrows). Both CD4-IgG- (n = 22) or EphA5-IgG-infused mice (n = 23) responded to training with increased freezing, a natural response to painful stimuli, and no significant differences were seen between groups. Relative duration (percentage; time per 60 sec) of freezing behavior is shown for 60 sec intervals. In addition to freezing, three other behavioral elements (bar graphs under line diagrams) are also shown. Note that fear correlates negatively with locomotion and grooming and positively with long-body. No significant differences were detected between the mice in any of the behavioral measures either before (interval 0-180 sec) or after (interval 180-360 sec) shock. B, A randomly assigned subset of trained mice (n = 16 for CD4-IgG-infused; n = 17 for EphA5-IgG-infused) was tested in the shock chamber for response to contextual stimuli. No tone cues or shocks were given. The freezing behavior (line diagram) of EphA5-IgG-infused mice was significantly impaired compared with that of the CD4-IgG-infused animals (F(1,31) = 24.926; p < 0.0001). In addition to freezing, relative duration of three other behavioral elements (bar graphs) is also shown for the entire session. EphA5-IgG-infused mice were found to exhibit an increased amount of locomotion (t = 4.315; df = 31; p < 0.0001) and grooming (t = 2.133; df = 31; p < 0.05) and exhibited decreased long-body posture (t = 2.100; df = 31; p < 0.05), all suggesting decreased level of fear. C, A randomly assigned subset of trained mice (n = 12 for CD4-IgG; n = 13 for EphA5-IgG) was tested in the cued test. The cued test was conducted in a chamber that lacked the olfactory, visual, and tactile cues (the contextual stimuli) of the shock chamber. Mice received three tone signals alone (solid horizontal bars) but no shock. Both groups of mice responded to the tone cue with a robust increase in freezing (line diagram), and no significant differences were found between the two groups of mice on freezing (F(1,23) = 2.068; p > 0.15) or any of the other behavioral measures (bar graphs) analyzed (t < 0.99; df = 23; p > 0.30). Data obtained in fear conditioning are shown as mean ± SEM.
It is unlikely that a context-specific learning deficit induced by the EphA antagonist may result from nonspecific disruption of brain function unrelated to learning. Nevertheless, to rule out this possibility, one may need to show improved learning performance in response to EphA activation. Thus, ephrinA5-IgG, the agonist immunoadhesin (Winslow et al., 1995
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Figure 6. Infusion of ephrinA5-IgG in DBA/2 mice improves spontaneous alternation rate in the T-maze (T-CAT paradigm). A, EphrinA5-IgG-treated mice (white bar; n = 19) exhibited higher levels of alternation compared with CD4-IgG-infused mice (black bar; n = 17; t = 2.85; df = 34; p < 0.01). B, Time spent to complete 15 alternation trials did not differ between treatment groups (t = 0.365; df = 34; p > 0.710), suggesting that the improved alternation performance is not caused by motoric or motivational influences. Error bars represent SEM. Methods as in Figure 4 (also see Materials and Methods).
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Figure 7. EphrinA5-IgG infusion significantly improves learning performance in a context-specific manner in fear conditioning in DBA/2 strain of mice. Methods are described in detail previously (Gerlai, 1998b
To investigate whether the improving effects of intrahippocampal ephrinA5-IgG infusion are generalizable to other mouse strains, we infused C57BL/6 mice with this immunoadhesin or the control CD4-IgG. Normal C57BL/6, or CD4-IgG-infused C57BL/6, mice exhibit good contextual and cue-dependent learning performance in fear conditioning (Gerlai, 1998b
The results of the one stimulus pair CDFC test convincingly demonstrated that ephrinA5-IgG improved performance in C57BL/6 mice in a context-dependent manner (Fig. 8). Figure 8A shows that all mice responded to a single tone-shock presentation with increased freezing, although the increase was less robust compared with when three such stimulus pairs were administered. Freezing response to context 1 d after training was at 30-40% level in the control CD4-IgG-infused mice (Fig. 8B), a performance similar to that reported previously in normal mice in this training paradigm (Silva et al., 1996
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Figure 8. EphrinA5-IgG infusion significantly improves learning performance in a context-specific manner in fear conditioning in C57BL/6 mice. Methods are described in detail previously (Silva et al., 1996
Gene expression changes induced by immunoadhesin infusion
Given the presynaptic and postsynaptic localization of EphA receptors (W.-Q. Gao et al., 1998
1), whose product is a cytosolic microtubular protein involved in dendritic and axonal cytoskeletal processes, showed significant immunoadhesin-induced changes. Tubulin mRNA expression tested by RT-PCR showed that EphA5-IgG increases and ephrinA5-IgG decreases transcription (Fig. 9A) from this gene, a finding consistent with the growth-arresting repulsive effects of the ephrin-A5 ligand during CNS development. Furthermore, another cytoskeletal protein, the microtubule-associated protein MAP2 involved in neuronal activity-dependent dendritic structural changes (Quinlan and Halpain, 1996
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Figure 9. Transcriptional changes induced by immunoadhesins in two cytoskeletal proteins, tubulin (A) and MAP2 (B). No strain differences were found. The data (mean ± SEM) are pooled for the strains and are based on the number of PCR amplification cycles required to reach a threshold cleavage level of fluorescent reporter probe18, 19. Results normalized to GAPDH housekeeping gene transcript are shown (
Immunoadhesin infusion alters synaptic plasticity
Hippocampal LTP is a cellular mechanism proposed to underlie spatial and configural learning in rodents (Bliss and Collingridge, 1993
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Figure 10. EphA5-IgG impairs LTP maintenance in hippocampal slices prepared from C57BL/6 mice. A, Field EPSP is expressed as percentage of baseline. Twenty sequential responses were averaged and plotted as one point. ANOVA revealed a significant immunoadhesin effect (F(1,8) = 8.09; p = 0.02) and a significant immunoadhesin × time interaction (F(29,232) = 4.98; p < 0.0001). Tukey's HSD test showed that the groups became significantly different (p < 0.05) 90 min after tetanization. Representative traces before and after tetanization at corresponding time points, as indicated, are also shown. B, No immunoadhesin effect was observed on paired pulse facilitation (F(1,11) = 0.164; p > 0.690), which was assessed by applying paired pulses of equivalent intensity at interpulse intervals as indicated. Facilitation ratios are calculated by expressing the slope of the second fEPSP as a percentage of the slope of the first fEPSP. C, Basal synaptic transmission, estimated by ratio of the fEPSP slope to the PSFV amplitude, was not altered by EphA5-IgG-infused (hatched bar) compared with CD4-IgG-infused (black bar) mice (t = 1.119; df = 14; p > 0.28). Estimation of basal synaptic transmission by I/O characteristics using Michaelis-Menten sigmoid curve fit revealed no significant differences (CD4-IgG, mean of 1.30 ± 0.368; EphA5-IgG, mean of 1.54 ± 0.219; p > 0.80).
The enhancement of cognitive function by ephrinA5-IgG infusion seen in DBA/2 mice was also accompanied by changes in hippocampal synaptic function. Slices from DBA/2 mice infused with ephrinA5-IgG exhibited a significant augmentation of LTP, beginning at induction and persisting up to 4.5 hr (Fig. 11A). EphrinA5-IgG treatment also increased PPF (Fig. 11B), suggesting the involvement of a presynaptic mechanism, whereas basal synaptic transmission was unchanged (Fig. 11C). Furthermore, although LTP induced by the standard four train stimulation protocol (see Materials and Methods) appeared almost identical in C57BL/6 mice infused with CD4-IgG or ephrinA5-IgG (immunoadhesin effect, F(1,8) = 0.043; p > 0.80; immunoadhesin × time interaction, F(30,240) = 0.917; p > 0.50), probably attributable to a robust LTP response leading to a ceiling effect, LTP induced by a single train and lower amplitude of electric stimulation showed a trend in C57BL/6 similar to the observations in DBA/2, suggesting a facilitatory effect of ephrinA5-IgG (Fig. 12) in both strains. It is notable, however, that although the electrophysiological and behavioral findings are generally in agreement with each other, the correlation is not perfect. For example, ephrinA5-IgG infusion was able to elicit a significant behavioral improvement in both DBA/2 and C57BL/6. This may be attributable to the genetic background of the two mouse strains differentially affecting behavioral and electrophysiological phenotypes and/or to different sensitivity and resolution of the electrophysiological and behavioral methods applied.
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Figure 11. EphrinA5-IgG improves LTP and increases magnitude of PPF in hippocampal slices prepared from DBA/2. A, Field EPSP expressed as percentage of baseline. Twenty sequential responses were averaged and plotted as one point. ANOVA, including data from all time points, revealed an immunoadhesin effect that bordered significance (F(1,12) = 4.23; p = 0.06), whereas Tukey's HSD test showed that the groups were significantly different (p < 0.05) up to 260 min post-tetanization. Representative traces before and after tetanization at corresponding time points, as indicated, are also shown. B, PPF varied as a function of immunoadhesin treatment (F(1,21) =6.189; p < 0.03), and no significant immunoadhesin × interval interaction (F(4,84) = 1.654; p > 0.16) was seen. C, No significant differences were found in basal synaptic transmission between ephrinA5-IgG-infused (white bar) and CD4-IgG-infused (black bar) mice (t = 0.416; df = 18; p > 0.68). Estimation of basal synaptic transmission by I/O characteristics using Michaelis-Menten sigmoid curve fit revealed no significant differences (CD4-IgG, mean of 2.49 ± 0.33; ephrinA5-IgG, mean of 2.80 ± 0.97; p > 0.70).
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Figure 12. Chronic ephrinA5-IgG infusion leads to an apparent increase of LTP in hippocampal slices prepared from C57BL/6 mice. Individual responses measured once every 30 sec are plotted. Open circles, EphrinA5-IgG infusion (n = 6); filled triangles, CD4-IgG infusion (n = 6). One hippocampal slice per experimental animal was tested; thus, n represents the number of animals analyzed. Error bars indicate SE. ANOVA revealed that the apparent immunoadhesin effect was not significant (F(1,10) = 1.973; p = 0.190) nor was the time × immunoadhesin interaction significant (F(60,600) = 0.447; p > 0.50).
DISCUSSION
Our in situ hybridization findings demonstrating strong EphA5 expression in neurons of the adult mouse hippocampus, RT-PCR results showing hippocampal expression of two relevant ligands of this receptor, ephrin-A2 and -A5, and our Western blot analysis revealing the presence of EphA5 receptor in a phosphorylated active form in hippocampal tissue from adult mice, strongly suggest that EphA receptor function is not restricted to the developing nervous system. Confirming this suggestion, intrahippocampal infusion of an EphA antagonist led to significant impairment in behavioral function in adult mice, whereas infusion of an agonist resulted in improved behavioral performance. Furthermore, infusion of the antagonist led to increased expression of a cytostructural protein, tubulin, and also impaired some electrophysiological measures of hippocampal synaptic plasticity, whereas infusion of the agonist resulted in decreased tubulin expression and improved electrophysiological performance.
These results were achieved using protein targeting, a novel strategy in behavioral neuroscience that may have some advantages over more conventional methods (Gerlai et al., 1998b
Our results indicate that inhibition and augmentation of EphA function by intrahippocampal infusion of the immunoadhesins in adult mice impairs and facilitates, respectively, behavioral responses in two tasks, T-CAT and CDFC. These tasks depend on the hippocampus (Gerlai, 1998a
The potential neurobiological mechanism underlying the observed behavioral effects is speculative at this point. The recent observation showing that Eph receptors and their ephrin ligands contain PDZ recognition motifs and are bound and clustered by PDZ proteins at presynaptic and postsynaptic sites of neuronal synapses in vitro suggests that Eph receptors may mediate synaptic plasticity (Hsueh and Sheng, 1998
EphA receptors may interact with a number of proteins through their PDZ binding domains that mediate cytoskeletal processes (Torres et al., 1998
The possibility that EphA receptors play roles in cytostructural processes is consistent with the changes we observed in the expression of tubulin gene in response to EphA5-IgG or ephrinA5-IgG treatment. Our results suggested that tubulin, a component of the cytoskeleton, was overexpressed in response to EphA receptor inactivation and was underexpressed in response to receptor activation in the adult mouse hippocampus, findings compatible with the known arresting effects of ephrin-A ligands on axonal and dendritic growth during CNS development (Winslow et al., 1995
An intriguing aspect of our findings is the observed cognitive improvement and facilitated LTP both induced by ephrinA5-IgG. LTP has been suggested to be a cellular mechanism that underlies learning and memory (Bliss and Collingridge, 1993
Regardless of the precise identity of the molecular and neurobiological mechanisms, the present findings now have revealed a role for EphA receptor tyrosine kinases in cognitive function in the adult mammalian brain. These findings open an unexpected avenue into the functional analysis of this large receptor protein family and may lead to novel targets for therapeutic intervention in human brain and behavioral disorders.
FOOTNOTES Received March 8, 1999; revised Aug. 20, 1999; accepted Aug. 20, 1999.
We thank Nerrisa Mendoza and Alisha Eisert for technical help; Louis Tamayo and Allison Bruce for figures; Steven Chamow for CD4-IgG; and Ingrid Caras, Nicola Clayton, Wim Crusio, and David Shelton for discussions on earlier versions of this manuscript.
Correspondence should be addressed to R. Gerlai, Mailstop #72, Room 10-413, 1 DNA Way, South San Francisco, CA 94080. E-mail: gerlai{at}gene.com.
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