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Previous Article | Next Article
Volume 17, Number 8, Issue of April 15, 1997 pp. 2876-2885
Copyright ©1997 Society for NeuroscienceSelective Alteration of Long-Term Potentiation-Induced Transcriptional Response in Hippocampus of Aged, Memory-Impaired Rats
Anthony Lanahan1, Gregory Lyford1, Gail S. Stevenson5, Paul F. Worley1, 2, and Carol A. Barnes3, 4, 5 Departments of 1 Neuroscience and 2 Neurology, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205-2185, and Departments of 3 Psychology and 4 Neurology, and 5 Division of Neural Systems, Memory and Aging, University of Arizona, Tucson, Arizona 85424
ABSTRACT
Normal human aging is associated with selective changes in cognition that are attributable, in part, to dysfunction of hippocampal pathways. Rodents also exhibit age-dependent hippocampal dysfunction that results in spatial memory deficits and a correlated reduction in the maintenance of long-term potentiation (LTP). Although suprathreshold stimulus protocols result in normal LTP induction in aged rats, the ability to sustain this increase in synaptic efficacy is reduced in the old animals. The maintenance phase of LTP is known to be dependent on rapid, transcriptional events, and recent studies have identified signal transduction mechanisms that link glutamate-induced responses at the synapse with transcriptional responses at the nucleus. To examine the integrity of these signaling pathways in aged hippocampus, we monitored the induction of a panel of immediate early genes (IEGs) that are known to be transcriptionally activated after LTP-inducing stimuli, using a "reverse Northern" strategy. Here we report that a broad representation of IEGs are similarly induced in awake, behaving young adult and aged, memory-impaired rats. This indicates a general preservation of these presumptive signaling pathways during the aging process. Induced levels of c-fos mRNA, however, are significantly higher in the aged animals. These observations suggest that age-dependent hippocampal dysfunction may be associated with a selective change in the dynamic activity of signaling pathways upstream of c-fos, possibly involving calcium regulation.
Key words: long-term potentiation (LTP); immediate early gene; aging; reverse Northern; age-dependent memory decline; transcription; protein synthesis inhibitor
INTRODUCTION
Rodents exhibit an age-dependent impairment of spatial learning that is correlated with a deficit in the maintenance of hippocampal long-term potentiation (LTP) (Bliss and Lomo, 1973
; Barnes, 1979
A primary question examined in the present experiment is whether alterations in signal transduction mechanisms could potentially contribute to memory deficits observed in old animals. Consistent with this hypothesis is the observation that the age-dependent decrease in LTP maintenance is not detectable for several days after robust induction protocols. The emergence of the age deficit at long time intervals argues strongly for mechanisms requiring macromolecular synthesis, because in all systems examined to date, LTP lasting >24 hr requires such synthesis. Moreover, in a number of systems, aging is known to be associated with changes in transcriptional mechanisms that result in altered cellular responses to tissue-specific signals (Ammendola et al., 1992
MATERIALS AND METHODS
Behavioral testing and stimulation protocols. Two age groups of male F-344 retired breeder rats were obtained from Charles River Laboratories at 9 and 26 months, respectively. When they were killed, the rats were 10 (n = 14) and 27 (n = 11) months, respectively. The Morris swim task (Morris, 1981
Behaviorally tested rats were then implanted surgically with recording electrodes [114 µm Teflon-coated stainless steel (Medwire Corp.)] in the hilus of the fascia dentata, and stimulating electrodes were implanted in the perforant pathway for chronic bilateral in vivo recordings of hippocampal population responses (Barnes and McNaughton, 1985
Control rats (n = 3; 4 months) were similarly pretreated with cycloheximide and received a maximal electroconvulsive seizure (MECS) from an electroconvulsive therapy (ECT) unit (Ugo Basile), as described previously (Worley et al., 1993
"Reverse Northern" analysis. Plasmids containing the indicated cDNAs were linearized with the appropriate restriction enzymes, and 1 µg of each plasmid was loaded per lane and electrophoresed in 1% agarose gels. Several identical gels were prepared and after denaturation and neutralization were transferred to nitrocellulose. Poly(A+)RNA was isolated from individual samples using micro Fastrack (Invitrogen, San Diego, CA), and nonradioactive double-stranded cDNA was synthesized using an oligo dT primer with Superscript reverse transcriptase (Life Technologies, Gaithersburg, MD) according to the manufacturer's protocol. Briefly, 5 µg of poly(A+)RNA was mixed with 1 µg of an oligo dT primer, heated at 70°C for 10 min, and cooled on ice. First-strand cDNA was synthesized in the presence of 50 mM Tris, pH 8.3, 7.5 mM KCl, 3 mM MgCl2, 10 mM dithiothreitol (DTT), 500 µM of each dNTP, 1 U/µl RNasin (Promega, Madison, WI), and 1000 U of SuperScript Reverse Transcriptase (Life Technologies). The final reaction mix of 20 µl was incubated at 40°C for 60 min. The single-stranded cDNA was converted to double-stranded by incubating at 16°C for 2 hr in the presence of 25 mM Tris, pH 7.5, 100 mM KCl, 5 mM MgCl2, 10 mM (NH4)2SO4, 0.15 mM B-NAD+, 250 µM of each dNTP, 1.2 mM DTT, 65 U/ml Escherichia coli DNA Ligase, 250 U/ml DNA polymerase I, and 13 U/ml RNase; the final reaction volume was 150 µl. The reaction was terminated by adding EDTA to 20 mM, and the reaction was extracted with phenol and precipitated with ethanol in the presence of 100 µg of glycogen. The precipitated cDNA mix was then chromatographed over a NICK column (Pharmacia, Piscataway, NJ) and reprecipitated in the presence of glycogen (100 µg) to remove free nucleotides that might hamper the [32P]dCTP radiolabeling of the cDNA. cDNA was radiolabeled by random priming (Pharmacia) with [32P]dCTP (NEN) to a specific activity of >109 cpm/µg. Identical blots were prehybridized overnight at 68°C in 5× SSC, 5× Denhardt's solution, 10 mM EDTA, 0.2% SDS, 50 mM NaPO4, pH 7.0, and 100 µg/ml boiled, sonicated salmon sperm DNA. Blots were then hybridized overnight in freshly prepared hybridization solution containing 1 × 106cpm/ml of the appropriate 32P-labeled cDNA probe (Lanahan et al., 1992 80°C for 1-3 d. Several of the IEGs used in this panel are novel and were identified by differential screening of cDNA libraries prepared from MECS-stimulated hippocampus as described previously (Yamagata et al., 1993
, and the reference describes their regulation in brain): glyceraldehyde phosphate dehydrogenase (GAPD);
-tubulin,
fos (Morgan et al., 1987
A activin (Andreasson and Worley, 1995
(Yamagata et al., 1994a
) (Gall and Lauterborn, 1992
-actin; activity-regulated cytoskeleton-associated protein (Arc; Lyford et al., 1995
Statistical analyses. For the behavioral analyses, two-way ANOVAs were used to test the main effects of age and trials (the latter to determine whether each group learned the tasks). For the comparisons of mRNA levels, two-way ANOVAs were used to test the main effects of age (AGE) and stimulation (STIM) and the interaction of AGE × STIM.
RESULTS
Reverse Northern analysis of multiple IEGs in small tissue samples
To compare induced mRNA levels in adult and aged rats in response to an LTP-inducing stimulus, it is experimentally advantageous to be able to assess responses in individual hippocampi. We therefore examined the feasibility of using a reverse Northern strategy. With this technique, levels of tissue mRNA are assessed by monitoring the intensity of hybridization signal of radiolabeled cDNA prepared from tissue RNA to Southern blots containing cloned cDNAs of multiple candidate IEGs (Lanahan et al., 1992
A critical step for the reverse Northern technique is the conversion of RNA to cDNA. This step is important both from the standpoint of obtaining sufficient material from small tissue samples and for achieving labeled probe that is representative of tissue mRNA levels. We prepared poly(A+)mRNA from individually dissected hippocampi and were routinely able to convert ~30% of poly(A+)RNA to first-strand cDNA. Copying the second strand of cDNA doubled this yield. Because the yield of poly(A+)RNA from a single hippocampus is typically ~1 µg, we are able to prepare ~600 ng of cDNA from a single hippocampus. To use this cDNA for differential Southern analysis, cDNA is labeled by random priming, which achieves a specific activity of ~2 × 109 dpm/µg cDNA. Approximately 50 ng of cDNA is sufficient to prepare probe for a 20 lane Southern blot using standard agarose gel chromatography and solution hybridization techniques. Accordingly, a single hippocampus is more than sufficient for this analysis. Note that all of these enzymatic steps are linear with respect to the tissue RNA concentrations, which ensures that the labeled cDNA is representative of the relative abundance of each species of mRNA in the tissue. No PCR step is used in the preparation of labeled cDNA.
In Figure 1, we use the reverse Northern to compare mRNA levels in hippocampus of control rats and rats that received a maximal MECS. MECS is a simple and reliable means to induce the expression of IEGs in the hippocampus, and it produces very robust and durable potentiation of the perforant pathway-granule cell synapse (Barnes et al., 1994 
Fig. 1. "Reverse northern" analysis of IEG induction by seizure. Duplicate Southern blots were probed with radiolabeled cDNA prepared from hippocampus of naive control (A) and MECS with cycloheximide-stimulated (B) rats.
[View Larger Version of this Image (29K GIF file)]
Analysis of LTP-induced IEG response by reverse Northern
We devised an LTP stimulation protocol that mimics the type of repetitive stimulus that results in age-dependent differences in LTP maintenance and also optimizes detection of IEGs. Age-dependent reductions in LTP maintenance have been observed after multiple (12), daily repetitions of standard LTP-inducing HF stimuli (i.e., time constant of decay for old = 17 d, for young = 37 d) (Barnes and McNaughton, 1980
In pilot studies, we identified a repetitive stimulation protocol that resulted in robust induction of mRNAs for the IEGs zif268 and jun B (12 repetitions of HF stimulus administered every 15 min; see Materials and Methods). cDNA was prepared from microdissected dorsal and ventral fascia dentata of the hippocampus of control and adult rats after LTP induction and was used to screen replicate Southern blots of a panel of 19 IEGs (Fig. 2B). Duplicate blots were also probed with cDNA from hippocampus of naive control and MECS-stimulated rats (Fig. 2A). Consistent with previous in situ hybridization studies (Worley et al., 1993 
Fig. 2. IEG induction by LTP stimulation in adult and aged hippocampus. Cloned cDNA inserts of a panel of IEGs were transferred to nitrocellulose and probed with radiolabeled cDNA prepared from individual hippocampi of naive young controls (top right), MECS-stimulated young controls (bottom right), LF-stimulated young and old rats (middle panels), and HF-stimulated young and old rats (left panels). The HF stimulus induced robust LTP (43 and 45% population response increase in young and old rats, respectively). Blots presented in the figure are qualitatively representative of the indicated population (n = 10 for young LF and HF; n = 8 for aged LF and HF). Note that MECS induces a robust increase in mRNA levels of nearly all the genes (19 IEGs) in the panel, whereas HF stimulation produces a more selective induction of IEGs in both young and old rats. c-fos mRNA (asterisk) is strongly induced by MECS and by the HF stimulus in aged rats but not young rats.
[View Larger Version of this Image (91K GIF file)]
Fig. 4. Comparison of IEG induction in young and old rats. Histograms comparing normalized (based on GAPD level) mRNA levels in fascia dentata induced by patterned HF stimulation in chronically implanted young adult and aged, memory-impaired rats. Levels of hybridization in low-frequency (LF)- and high-frequency (HF)-stimulated fascia dentata were quantitated as described in Materials and Methods. Two-way ANOVA indicates that c-fos mRNA is significantly induced in anterior hippocampus (A) by the HF stimulus in both young and old rats (F1,32 = 45.246; p < 0.0001), and the induction is greater in the aged animals than in the young adults (F1,32 = 9.409; p = 0.0044). The interaction between age and LTP is also significant (F1,32 = 6.157; p = 0.0185). zif268 and jun B were similarly induced by the HF stimulus in young and old rats, whereas Fra-1 was not induced in either young or old rats (for statistics, see Results). As an additional control, we examined c-fos mRNA levels in the posterior one third of the hippocampi (B), in which we demonstrated previously that IEGs are not induced by HF stimulation, using standard electrode placements (Barnes et al., 1994
[View Larger Version of this Image (13K GIF file)]
Comparison of behavioral performance and LTP-induced IEG responses in adult and aged rats
cDNA was prepared from individual fascia dentata of young adult and old rats after LF (0.1 Hz) or HF (400 Hz) stimuli in the awake, freely behaving state (see Materials and Methods). As observed in previous studies (Gallagher et al., 19932 = 11.59; p < 0.001). The performance of the old rats, however, did not differ from that of the young rats when the platform was not submerged and a distinct visual cue was suspended above it (F1,19 0.13; p = 0.72), and both young and old rats showed improvement over trials (F1,19 2.68; p = 0.026).
Fig. 3. A, Mean ± SEM corrected integrated path length (CIPL; see Materials and Methods) over 4 d (six trials per day) of training in the spatial version of the Morris swim task. The old rats took significantly longer paths to find the platform compared with the young rats on days 2, 3, and 4 of training. B, Mean ± SEM CIPL for six training trials on the visual discrimination version of the Morris swim task. There were no statistically significant differences between age groups. C, Mean ± SEM average distance to the target quadrant and target crossings during the spatial probe trial, in which the platform was removed from the pool. The old rats exhibited longer average distances to the target and fewer target crossings than did the young rats, suggesting poorer spatial performance accuracy in the old animals.
[View Larger Version of this Image (33K GIF file)]
Reverse Northern blots were performed to compare induced IEGs. A qualitative comparison of 10 young rats and 8 aged rats illustrated similar robust inductions of the same IEGs by the HF stimulus in young and old rats (compare Fig. 2, B and C). This analysis suggested additionally that certain of the IEGs might be induced to different extents in young and aged rats. Accordingly, we performed a quantitative analysis of responses using a phosphorimager. To reduce the complexity of the analysis, we focused on a set of five IEGs that are induced in association with LTP.
Normalized IEG mRNA levels in the anterior two thirds and posterior one third of the hippocampus were subjected to a two-way ANOVA to test the main effects of age (AGE) and stimulation (STIM) and the interaction of AGE × STIM (Table 1, Fig. 4). In the anterior hippocampus, normalized mRNA levels for c-fos revealed significant effects for AGE and STIM as well as a significant interaction of AGE × STIM. Similar analyses for jun B, c-jun, and zif268 mRNA levels revealed significant effects of STIM but no significant effects for AGE or AGE × STIM. Analysis of anterior hippocampal fosB and fra1 mRNA levels revealed no significant effects. Similar analysis of posterior hippocampal mRNA levels demonstrated no significant effects for all genes analyzed. Analysis of posterior zif268 mRNA levels was not conducted because of insufficient sample size.
Table 1. Results of two-way ANOVA of mRNA
Anterior hippocampus Posterior hippocampus Age STIM Age × STIM Age STIM F P F P F P F P F P c-fos 9.41 <0.01 45.25 <0.01 6.16 <0.05 0.03 0.87 0.07 0.81 jun B 3.68 0.06 19.45 <0.01 2.26 0.14 0.06 0.82 1.29 0.29 c-jun 3.46 0.07 9.95 <0.01 0.29 0.60 0.18 0.68 2.36 0.16 fos B 1.90 0.17 1.42 0.24 - - 0.60 0.46 0.00 0.98 fra1 0.41 0.53 1.53 0.22 - - 0.49 0.50 0.68 0.43 zif268 0.48 0.49 40.13 <0.01 1.53 0.23 - - - - Separate analyses of mRNA levels from anterior two thirds and posterior one third of hippocampus were performed for the factors AGE (young vs old) and STIM (low frequency vs high frequency). Degrees of freedom for all genes analyzed in anterior hippocampus were (1,32), except for zif268 which was (1,19). In the analysis of posterior mRNA levels, degrees of freedom were (1,9).
DISCUSSION
The present study demonstrates that the IEG response to patterned HF synaptic activity is largely intact in the senescent hippocampus. The stimulation paradigm that we have developed, which combines repetitive stimulation in the presence of protein synthesis inhibition, faithfully reproduces the pattern of gene activation seen using conventional in situ and Northern techniques after HF stimulation and boosts levels of induced mRNAs, thereby markedly improving the sensitivity of their detection. Application of the reverse Northern strategy amplifies the number of genes that can be monitored with small tissue samples.
Our survey included a large panel of IEGs and is anticipated to test the functional integrity of signaling and transcriptional mechanisms that control the expression of these genes. We infer that the age-dependent deficit of LTP maintenance is not attributable to a general disruption of these signaling pathways. This result stands in contrast to the reported age-dependent changes in second messenger pathways that are likely be involved in the transduction of extracellular signals into transcriptional responses. For example, aging is associated with reductions in phosphoinositide metabolites and protein kinase C activation (Martini et al., 1994
Despite the general conservation of IEG induction in aged rats, quantitative comparisons with adult rats indicate an increase in induced levels of c-fos mRNA in aged animals. c-fos mRNA and protein have been examined previously in aged rodents in response to various stimuli. c-fos is reported to show reduced inducibility in the suprachiasmatic nucleus of aged rats in response to visual stimulation (Sutin et al., 1993
We have previously demonstrated distinct thresholds for the synaptic activation of different IEGs (Worley et al., 1993
The transcriptional regulation of c-fos involves multiple regulatory elements and binding proteins, including CRE/CREB, AP-1, SIE/SIF (p91), and SRE/SRE binding protein (Treisman, 1985
The present study provides an assay of a dynamic function of the hippocampus that is relevant to age-dependent memory decline and focuses attention on specific cellular mechanisms that regulate the response of c-fos. One caveat regarding the reverse Northern strategy, in its present use, is that it lacks cellular resolution, and it remains to be determined whether age-dependent changes in gene expression after the LTP-inducing stimulus are uniquely associated with neurons. It has recently become possible to assay mRNA in single neurons (Crino and Eberwine, 1996
FOOTNOTES
Received Oct. 9, 1996; revised Jan. 17, 1997; accepted Jan. 31, 1997.
This work was supported by Public Health Service Grants AG09219 (C.B., P.W.), MH01152 (P.W.), and MH01227 (C.B.). We thank L. Church and G. Rao for assistance with these experiments.
Correspondence should be addressed to Dr. P. F. Worley, Department of Neuroscience, Johns Hopkins University School of Medicine, 725 N. Wolfe Street, Baltimore, MD 21205-2185.
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