Protein Synthesis Inhibition Blocks the Late-Phase LTP of C-Fiber Evoked Field Potentials in Rat Spinal Dorsal Horn

doi:10.1152/jn.01027.2002

Protein Synthesis Inhibition Blocks the Late-Phase LTP of C-Fiber Evoked Field Potentials in Rat Spinal Dorsal Horn

Neng-Wei Hu, Hong-Mei Zhang, Xiao-Dong Hu, Ming-Tao Li, Tong Zhang, Li-Jun Zhou, and Xian-Guo Liu

Department of Physiology, Zhongshan Medical School of Sun Yat-sen University, 74 Zhongshan Rd 2, Guangzhou 510089, People's Republic of China

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Hu, Neng-Wei, Hong-Mei Zhang, Xiao-Dong Hu, Ming-Tao Li, Tong Zhang, Li-Jun Zhou, and Xian-Guo Liu. Protein Synthesis Inhibition Blocks the Late-Phase LTP of C-Fiber Evoked Field Potentials in Rat Spinal Dorsal Horn. J. Neurophysiol. 89: 2354-2359, 2003. Previous studies have demonstrated that in the hippocampus the maintenance of long-term potentiation (LTP) requires de novoprotein synthesis. To investigate the role of protein synthesisin the maintenance of LTP of C-fiber evoked field potentials inspinal dorsal horn, which may be relevant to hyperalgesia, proteinsynthesis inhibitor (either cycloheximide or anisomycin) was appliedlocally to the recording segments of spinal cord in anesthetizedrats, 30 min prior to tetanic stimulation to the sciatic nerve.We found that both cycloheximide and anisomycin selectively inhibitedlate-phase maintenance of the spinal LTP but affected neitherLTP induction nor baseline responses of C-fiber evoked field potentials.In the presence of cycloheximide, LTP of C-fiber evoked fieldpotentials was 281.5 ± 16.5% (n = 6) of baseline 1 h after tetanicstimulation and the potentiation significantly decreased to 235.5± 18.5% at 145 min after tetanic stimulation (P < 0.05). Afterward,LTP of C-fiber evoked field potentials decreased continuouslyand at 270 min after tetanic stimulation reached 130.8 ± 18.0%,which was no longer different from baseline (P > 0.05). Spinalapplication of anisomycin at 30 min before tetanic stimulationyielded similar results (n = 6). These results suggest that proteinsynthesis may be crucial for the late-phase maintenance of LTPof C-fiber evoked field potentials in spinal dorsalhorn.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Long-term potentiation (LTP), which is first described in the hippocampus (Bliss and Lomo 1973), refers to a long-lastingenhancement in efficacy of synaptic transmission and is believedto be a synaptic model of learning and memory (Bliss and Collingridge1993). Besides the hippocampus, LTP has been also found in severalother parts of nervous system. Some of them may be relevant topathological processes (McEachern and Shaw 1999).

In response to intensive noxious stimulation, neurons in spinal dorsal horn become hypersensitive to subsequent stimuli (Maand Woolf 1995; Woolf 1983). The phenomenon that is termed centralsensitization is considered as a central mechanism underlyinghyperalgesia, an increased response to noxious stimuli (Woolfand Salter 2000). Just like hyperalgesia, LTP of C-fiber evokedfield potentials in spinal dorsal horn can be induced by electricalstimulation of afferent C-fibers (Liu and Sandkühler 1995, 1997),natural noxious stimulation on peripheral tissue, or acute nerveinjury (Sandkühler and Liu 1998). Accordingly, the spinal LTPis believed to be an attractive cellular model of injury-inducedhyperalgesia (Sandkühler 2000).

In the hippocampus two forms of LTP have been characterized. One is N-methyl-D-aspartate (NMDA) receptor-dependent (Harriset al. 1984; Hernandez et al. 1994) and another is NMDA receptor-independent(Harris and Cotman 1986). The maintenance of NMDA receptor-dependentLTP is divided into two phases, an early-phase (1-3 h) and a late-phase(>3 h). It has been well established that the late phase but notthe early phase of NMDA receptor-dependent LTP is protein synthesis-dependent(Bliss and Collingridge 1993; Frey et al. 1988; Krug et al. 1984).In the case of NMDA-independent LTP, the role of protein synthesisappears complicated. It has been shown that protein synthesisinhibitors selectively inhibit the late-phase maintenance of LTPin mossy fiber-CA3 synapses in vitro (Huang et al. 1994) but blockinduction of LTP in the same synapses in vivo (Barea-Rodriguezet al. 2000). LTP of C-fiber evoked field potentials in spinaldorsal horn is also NMDA receptor-dependent (Liu and Sandkühler1995). But the roles of protein synthesis in the induction andthe maintenance of the spinal LTP have not been established todate.

In the present work two protein synthesis inhibitors, cycloheximide and anisomycin, were tested. We found that both of themselectively inhibited the late-phase of LTP of C-fiber evokedfield potentials but did not affect its induction, when appliedlocally onto spinal dorsal horn at recording segments 30 min priorto LTPinduction.

	METHODS

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Surgical preparation

Adult male Sprague-Dawley rats (250-300g) were anesthetized with urethane (1.5 g/kg ip). The trachea was cannulated and theanimal breathed spontaneously. A catheter was inserted into oneexternal jugular vein for intravenous infusion of Tyrode's solutionat a rate of 0.8-1 ml/h. The caudal artery was cannulated to continuouslymonitor blood pressure, which was maintained at 80 to 120 mmHg.A laminectomy was performed to expose the lumbar enlargement ofthe spinal cord. The left sciatic nerve was dissected free forelectrical stimulation with silver chloride hook-electrodes. Therats were placed in a stereotaxic frame. All exposed nerve tissueswere covered with warm paraffin oil in a pool made of skin flaps,except for those spinal segments onto which the drug was applied.The body temperature of the rats was maintained at 37-38° witha feedback-controlled heating blanket. At the end of the experiments,animals were killed with an overdose of urethane. All experimentswere approved by the local animal carecommittee.

Measurement of evoked potentials

The electrophysiological recording of C-fiber evoked field potentials has been described elsewhere (Liu and Sandkühler 1995,1997). Briefly, following electrical stimulation of the sciaticnerve with a bipolar silver chloride hook-electrode, field potentialswere recorded with a tungsten microelectrode (impedance 0.5-1M $Omega$ ), which was driven by an electronically controlled microsteppingmotor (Narishige Scientific Instrument Laboratory) at a depthof 100-500 µm from the surface of the spinal cord in lumbar enlargement(L4 and L5 segments). An A/D converter card (DT2821-F-16SE, DataTranslation Inc.) was used to digitize and store data in a Pentiumcomputer at a sampling rate of 10 kHz. Single square pulses (0.5ms duration, delivered every 1 min) delivered to the sciatic nervewere used as test stimuli. The strength of stimulation was adjustedto 1.5-2 times the threshold for C-fiber response. A tetanic stimulation(100 Hz, 40 V, 0.5 ms, 100 pulses given in 4 trains of 1-s durationat 10-s intervals) was used to induce LTP of C-fiber evoked fieldpotentials. The distance from stimulating site at the sciaticnerve to the recording site in the lumbar spinal cord was approximately11cm.

Experiments were performed in four groups of rats. The first one was the drug and tetanus-treated group, in which either cycloheximide(n = 6) or anisomycin (n = 6) was applied onto the surface ofspinal cord at the recording segments, and 30 min later a tetanicstimulation was delivered. The second one was the drug controlgroup, in which cycloheximide (n = 5) or anisomycin (n = 5) wasgiven but no tetanic stimulation was delivered. The third wasthe vehicle and tetanus-treated group (n = 5). In this group salinewas applied 30 min before tetanic stimulation. In the fourth group(n = 6) only saline was applied but no tetanic stimulation wasdelivered (saline controlgroup).

Compounds and drug treatment

Cycloheximide (Sigma) was dissolved in 0.9% NaCl at concentration of 20 µg/µl. Anisomycin (2.4 mg, Sigma) was first dissolvedin 15 µl of 1 N HCl solution and then treated with 1 N NaOH toa pH of 7.0. The solution was subsequently diluted with 0.9% NaClto a concentration of 12 µg/µl. To perform the controlled superfusionof spinal cord, a small well on the cord dorsum at the recordingsegments was formed with 1.5% agar dissolved with normalsaline.

Data analysis

The area of C-fiber evoked field potentials was determined off-line by parameter extraction (see Fig. 1C), which was implementedby DataWave. In each experiment responses to five consecutivetest stimuli were averaged. The mean area of C-fiber evoked fieldpotentials before drug or saline application served as baseline.All data are expressed as means ± SE. For statistical analysis,data within animals were compared with the nonparametric Friedmantest and Wilcoxon signed-rank test and data between animals werecompared with Kruskal-Wallis test and Mann-Whitney U test, whenappropriate. Nonparametric tests were performed because the datafrom some groups were not normally distributed. P < 0.05 was consideredsignificant.

	RESULTS

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Saline affected neither spinal LTP nor baseline of synaptic transmission

Our previous work (Liu and Sandkühler 1997) has shown that tetanic stimulation of the sciatic nerve induces LTP of C-fiberevoked field potentials in spinal dorsal horn, which lasts untilthe end of the experiment ( $<=$ 10 h after tetanic stimulation), whenthe recording segments of the spinal cord are covered with warmparaffin oil. Because the protein synthesis inhibitors used inthe present study were dissolved in saline, we first tested whethersaline by itself could affect LTP of C-fiber evoked field potentialsor baseline synaptic transmission over a long period of recordingtime. In five rats the stable baseline of C-fiber responses wasrecorded for $>=$ 30 min and then saline (150 µl in volume) was applieddirectly onto the dorsal surface of the recording segments. Thirtyminutes later a tetanic stimulation (40 V, 0.5 ms, 100 Hz) wasdelivered to the sciatic nerve. As observed in previous work,the tetanic stimulation induced a robust LTP of C-fiber evokedfield potentials in every experiment. The potentiation was 268.8± 20% (P < 0.05, Wilcoxon signed ranks test, Fig. 1A) as measured1 h after tetanic stimulation and lasted until end of each experiment(for $>=$ 6 h after tetanic stimulation). In five other rats we observedthat spinal application of saline (without tetanic stimulation)had no effect on the basal synaptic transmission throughout thetime of the experiment (P > 0.05, Friedman test, Fig. 1B).

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Fig. 1. Spinal application of saline affects neither spinal long-term potentiation (LTP) (A) nor baseline response of synaptic transmission (B). In each experiment the C-fiber responses recorded before saline application were averaged and served as baseline. Mean area of C-fiber evoked field potentials, expressed as a percentage of baseline, was plotted versus time. Vertical bars indicate SEs. Downward arrows indicate the onset of saline application on the surface of spinal dorsal horn at recording segments and upward arrow represents the time of tetanic stimulation (100 Hz, 40 V, 0.5 ms, 100 pulses given in 4 trains of 1-s duration at 10-s intervals). C: representative original recordings taken at the time points as indicated. Area of C-fiber evoked field potential (b; filled with oblique lines) is determined automatically by parameter extraction. Baseline (dashed line) is determined by two highest points within the time range that is defined manually on either side of C-fiber response (arrowheads). Therefore a small change in latency of C-fiber evoked field potentials does not affect the measurement of the area.

Both cycloheximide and anisomycin selectively inhibit the late-phase of spinal LTP with no effect on LTP induction and baseline of synaptic transmission

In six rats cycloheximide (20 µg/µl, 150 µl in volume) was applied directly onto the recording segments following $>=$ 30 minstable recordings of C-fiber evoked field potentials. The applicationdid not affect LTP induction by a tetanic stimulation (100 Hz,40 V, 0.5 ms) delivered 30 min after the drug application. Onehour after tetanic stimulation, the mean potentiation in the sixrats was 281.5 ± 16.5% (P < 0.05, Wilcoxon signed-rank test, Fig.2A), which was not different compared with that recorded in salinegroup (268.8 ± 20%, P > 0.05, Mann-Whitney U test), indicatingthat the drug does not affect the spinal LTP induction and itsearly phase maintenance. However, the spinal LTP in this groupdecreased with time. At 145 min after tetanic stimulation, LTPdecreased to 235.0 ± 18.5%, which was significantly lower comparedwith that at 60 min after tetanic stimulation in the same groupof rats (P < 0.05, Wilcoxon signed-rank test) and was also significantlylower compared with that in the saline and tetanus-treated group(293.9 ± 15.5%, P < 0.05, Mann-Whitney U test, Fig. 3A), but stillsignificantly higher compared with baseline (P < 0.05, Wilcoxonsigned ranks test) and that in the drug control group describedbelow (P < 0.05, Mann-Whitney test, Figs. 2 and 3A). This suggestedthat at this time point the spinal LTP was substantially depressedbut did not reach baseline level yet. At 270 min after tetanicstimulation, LTP decreased to 130.8 ± 18.0%, which was no longerdifferent from baseline (P > 0.05, Wilcoxon signed-rank test)and was also not different compared with that recorded in thedrug control group (104.8 ± 4.8%, P < 0.05, Mann-Whitney U test,Figs. 2 and 3A), indicating the spinal LTP was not totally reverseduntil this time point.

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Fig. 2. Cycloheximide selectively inhibits the late phase of LTP of C-fiber evoked field potentials but affects neither the induction of the spinal LTP nor baseline response of C-fiber evoked field potentials. In each experiment the mean response recorded before drug application served as baseline. Mean area of C-fiber evoked field potentials, expressed as a percentage of baseline, was plotted versus time. Vertical bars indicate SEs. Downward arrows indicate the onset of drug application. Upward arrow represents the time of tetanic stimulation (100 Hz, 30-40 V, 0.5 ms). A: cycloheximide (CHX, 20 µg/µl) does not influence the LTP induction but inhibits the late-phase maintenance of the spinal LTP. B: cycloheximide (20 µg/µl) has no effect on the baseline response of C-fiber evoked field potentials throughout the experiment period. C: representative original recordings taken at the time points as indicated.

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Fig. 3. Effects of saline, cycloheximide, or anisomycin on the maintenance of LTP of C-fiber evoked field potentials and basal synaptic transmission. A: at 145 min after tetanic stimulation, the spinal LTP in the cycloheximide and tetanus-treated group (CHX + Tet) significantly decreased compared with that recorded in the saline and tetanus-treated group (Saline + Tet), indicating a substantial depression of the spinal LTP. But it was still higher than that recorded in cycloheximide control group (CHX). At 270 min after tetanic stimulation, the mean area of C-fiber evoked field potentials was no longer different from that in the cycloheximide control group, indicating a total reversal of the spinal LTP. B: a significant depression of the spinal LTP in anisomycin and tetanus-treated group (ANI + Tet) was observed at 125 min after tetanic stimulation and at 295 min after tetanic stimulation the mean area of C-fiber evoked field potentials reached baseline. Vertical bars indicate SEs. ^*P < 0.05.

In five other rats the same dosage (20 µg/µl, 150 µl in volume) of cycloheximide was administrated to the spinal cord following $>=$ 30 min stable baseline recordings. Recordings continued for $>=$ 7h without tetanic stimulation. The drug had no significant effecton the spinal basal synaptic transmission compared with the salinecontrol group (P > 0.05, Kruskal-Wallis test, Figs. 1B and 2B).

To exclude the possibility that cycloheximide may inhibit spinal LTP through nonspecific effects other than inhibition ofprotein synthesis, we next examined the effect of anisomycin,another translation inhibitor on spinal LTP in six other rats.When anisomycin (12 µg/µl, 150 µl in volume) was applied to thespinal cord 30 min before tetanic stimulation, a significant inhibitionof spinal LTP also occurred, which was similar to that found withcycloheximide (Fig. 4A). At 60 min after tetanic stimulation,potentiation was 261.9 ± 10% (P < 0.05, Wilcoxon signed-rank test),which was not different from that in the saline and tetanus-treatedgroup (P > 0.05, Mann-Whitney U test). At 125 min after tetanicstimulation, the spinal LTP decreased to 241.5 ± 9%, which wassignificantly lower compared with that recorded at 1 h after tetanicstimulation in the same group of rats (P < 0.05, Wilcoxon signed-ranktest) and was also significantly lower than that in the salineand tetanus-treated group (287 ± 17.6%, P > 0.05, Mann-WhitneyU test, Fig. 3B). But the value was still higher than baseline(P < 0.05, Wilcoxon signed-rank test) and also higher than thatrecorded in the drug control group (118.7 ± 8.5%, P < 0.05, Mann-Whitneytest, Fig. 3B). Until 295 min after tetanic stimulation the potentiationwas totally reversed, since the mean area of C-fiber evoked fieldpotentials decreased to 127.7 ± 15.3%, which was not differentfrom baseline (P > 0.05, Wilcoxon signed-rank test) and from thatrecorded in the drug control group (111.1 ± 6.4%, P > 0.05, Mann-WhitneyU test, Fig. 3B).

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Fig. 4. Anisomycin selectively inhibits the late-phase of LTP of C-fiber evoked field potentials but affects neither the induction of the spinal LTP nor baseline response of C-fiber evoked field potentials. A: anisomycin (ANI, 12 µg/µl) was applied on the surface of the spinal cord (downward arrow) and tetanic stimulation (100 Hz, 30-40 V, 0.5 ms) to the sciatic nerve was delivered 30 min later. B: spinal application of anisomycin (12 µg/µl) does not affect baseline response of C-fiber evoked field potentials. C: representative original recordings taken at the time points as indicated.

The same dosage (12 µg/µl, 150 µl in volume) of anisomycin applied to recording segments had no significant effect on C-fiberevoked field potentials compared with the effect in the salinecontrol animals. (P > 0.05, Kruskal-Wallis test, Figs. 1B and4B). Thus the spinal application of anisomycin did not affectthe baseline of synaptictransmission.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We found that inhibition of de novo protein synthesis by spinal application of cycloheximide or anisomycin before tetanicstimulation selectively inhibited the late-phase maintenance ofLTP of C-fiber evoked field potentials but did not affect theinduction and early-phase maintenance of the spinalLTP.

The results in the saline-treated group showed that LTP of C-fiber evoked field potentials induced by tetanic stimulationwas stable until end of the experiments ( $<=$ 6 h, Fig. 1A). Whenno tetanic stimulation was delivered, the baseline responses ofC-fiber evoked field potentials did not change during the wholerecording period (Fig. 1B). These indicate that our experimentmodel is suitable to investigate the late phase of the spinalLTP.

The unspecific effects of the drugs may be not responsible for the present results, because both cycloheximide and anisomycinblocked late phase of the spinal LTP in the same manner, evenwith a similar time course. It is well known that the two drugshave a common effect, protein synthesis inhibition, but theirside effects may be different. It has been reported that anisomycincan also strongly activate the mitogen-activated protein kinasesubtypes (Cano et al. 1994; Hazzalin et al. 1998), while the significantside effect of cycloheximide has not been documented. We believethat the inhibitory effect observed in the present study is attributableto inhibition of protein synthesis in spinal recordingsegments.

It is unlikely that the drugs at the dosages used in the present work may depress the spinal LTP maintenance by toxic effectsduring the long experimental time course, because we showed thatcycloheximide or anisomycin at the concentrations capable of inhibitingLTP maintenance did not affect basal synaptic transmission elicitedby test stimuli (Figs. 2B and 4B).

In the hippocampus, the late phase (>3 h) but not early phase (1-3 h) of NMDA receptor-dependent LTP depends on new proteinsynthesis (Frey et al. 1988; Krug et al. 1984; Mochida et al.2001). The present work demonstrated that the situation was verysimilar in spinal dorsal horn. In the presence of cycloheximideor anisomycin, a significant depression of LTP of C-fiber evokedfield potentials could be detected around 2 h after tetanic stimulation,and a complete reversal of the spinal LTP was observed around4 h after tetanic stimulation (Fig. 3). Unlike the LTP mentionedabove, the induction of some forms of long-lasting enhancementof synaptic transmission is protein synthesis-dependent, for instance,LTP induced by brain-derived neurotrophic factor and neurotrophin-3in hippocampus slices (Kang and Schuman 1996), the LTP in hippocampalmossy fiber-CA3 synapses induced by tetanic stimulation (Barea-Rodriguezet al. 2000), the long-term facilitation (LTF) in spinal respiratorymotor output induced by intermittent hypoxia (Baker-Herman andMitchell 2002), and the LTF of synaptic transmission in culturedAplysia sensory to motor neurons produced by repetitive applicationof serotonin (Martin et al. 1997). It has been proposed that LTPinitiates the creation of a short-lasting (<3 h) protein synthesis-independentsynaptic tag, and the tagged synapses can capture the proteinsthat are synthesized in soma and exported throughout the cell.In this way, newly synthesized proteins, which are crucial forlate-phase LTP, are transported and specifically targeted to thesynapses that are stimulated during LTP induction (Frey and Morris1997). This theory may explain the fact that the late-phase butnot the early-phase of LTP is inhibited by protein synthesis inhibitors(Frey and Morris 1998). Another source of new proteins is locallyat the synaptic sites. It has been demonstrated that synapse-associatedpolyribosome complexes are selectively localized beneath postsynapticsites on the dendrites of CNS (Steward and Levy 1982). The translationmachinery may synthesize key molecular constituents of the synapsein response to activation of synapse (Steward et al. 2001). Theproteins synthesized in dendrites are believed to contribute tothe induction or early-phase maintenance of some forms of LTP(Barea-Rodriguez et al. 2000; Kang and Schuman 1996). It is likelythat proteins synthesized in the cell body and in dendrites mayplay different roles in LTP maintenance. It has been shown thatthe $alpha$ -subunit of calcium/calmodulin-dependent protein kinase II(CaMKII) is synthesized in the dendrites (Scheetz et al. 2000)and activation of CaMKII is proved to be necessary for inductionbut not for maintenance of LTP in the hippocampus (Lisman et al.2002). Our unpublished data showed that CaMKII inhibitor (KN-93)blocked induction of LTP of C-fiber evoked field potentials whenapplied before LTP induction and reversed the established spinalLTP in a time-dependent manner. Within 1 h after LTP induction,KN-93 reversed LTP completely, but did not affect LTP when applied3 h after LTP induction, suggesting that early phase but not latephase of the spinal LTP may depend on the activation of CaMKII.The new proteins involved in the late-phase maintenance of thespinal LTP remain to beelucidated.

It is generally accepted that LTP in the hippocampus, a brain structure associated with memory (Scoville and Milner 1957),is a synaptic model of learning and memory (Bliss and Collingridge1993). In recent years different forms of LTP in spinal dorsalhorn have been demonstrated both in vivo (Liu and Sandkühler1995; Svendsen et al. 1999) and in vitro (Randic et al. 1993).It is well established that nociceptive A $delta$ - and C-fibers makethe first synaptic contact with neurons in the spinal dorsal horn(Gobel and Falls 1979; Gobel et al. 1981; Light and Perl 1979).Therefore the spinal LTP mediated by afferent A $delta$ - or C-fibersis suggested as a synaptic model for pain memory, which may berelevant to central sensitization, a central component of hyperalgesia(Liu and Sandkühler 1997; Melzack et al. 2001; Sandkühler 2000;Zimmermann 2001). This hypothesis is strongly supported by thefact that acute injury of the sural nerve or intensive noxiousstimulation of peripheral tissues induces the spinal LTP in spinalizedrats (Sandkühler and Liu 1998). Our recent work (in preparation)further demonstrates that acute injury of the sciatic nerve producesthe spinal LTP in intact rats. Furthermore, we have shown thatLTP-inducing tetanic stimulation delivered to the sciatic nerveproduces mechanical and thermal hyperalgesia that lasts for severaldays (Zhang et al. 2002). The new proteins synthesized duringLTP induction may play a role in the long-lasting abnormal painbehaviors.

	ACKNOWLEDGMENTS

This work was supported by the National Science Foundation of China (No. 30070256) and by China Medical Board-Sun Yat-senUniversity of Medical Sciences Scholar (98-766).

	FOOTNOTES

Address for reprint requests: X.-G. Liu (E-mail: xgliu{at}gzsums.edu.cn).

REFERENCES

TOP
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METHODS
RESULTS
DISCUSSION
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				J. W. Grau, E. D. Crown, A. R. Ferguson, S. N. Washburn, M. A. Hook, and R. C. Miranda Instrumental learning within the spinal cord: underlying mechanisms and implications for recovery after injury. Behav Cogn Neurosci Rev, December 1, 2006; 5(4): 191 - 239. [Abstract] [PDF]

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				H.-W. Yang, X.-D. Hu, H.-M. Zhang, W.-J. Xin, M.-T. Li, T. Zhang, L.-J. Zhou, and X.-G. Liu Roles of CaMKII, PKA, and PKC in the Induction and Maintenance of LTP of C-Fiber-Evoked Field Potentials in Rat Spinal Dorsal Horn J Neurophysiol, March 1, 2004; 91(3): 1122 - 1133. [Abstract] [Full Text] [PDF]

				C. Gao, H. Guo, L. Downey, C. Marroquin, J. Wei, and P. C. Kuo Osteopontin-dependent CD44v6 expression and cell adhesion in HepG2 cells Carcinogenesis, December 1, 2003; 24(12): 1871 - 1878. [Abstract] [Full Text] [PDF]

Protein Synthesis Inhibition Blocks the Late-Phase LTP of C-Fiber Evoked Field Potentials in Rat Spinal Dorsal Horn

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