Abstract
We have reported recently a high density of transient A-type K+ channels located in the distal dendrites of CA1 hippocampal pyramidal neurons and shown that these channels shape EPSPs, limit the back-propagation of action potentials, and prevent dendritic action potential initiation (Hoffman et al., 1997). Because of the importance of these channels in dendritic signal propagation, their modulation by protein kinases would be of significant interest. We investigated the effects of activators of cAMP-dependent protein kinase (PKA) and the Ca2+-dependent phospholipid-sensitive protein kinase (PKC) on K+ channels in cell-attached patches from the distal dendrites of hippocampal CA1 pyramidal neurons. Inclusion of the membrane-permeant PKA activators 8-bromo-cAMP (8-br-cAMP) or forskolin in the dendritic patch pipette resulted in a depolarizing shift in the activation curve for the transient channels of ∼15 mV. Activation of PKC by either of two phorbol esters also resulted in a 15 mV depolarizing shift of the activation curve. Neither PKA nor PKC activation affected the sustained or slowly inactivating component of the total outward current. This downregulation of transient K+ channels in the distal dendrites may be responsible for some of the frequently reported increases in cell excitability found after PKA and PKC activation. In support of this hypothesis, we found that activation of either PKA or PKC significantly increased the amplitude of back-propagating action potentials in distal dendrites.
- potassium channels
- IK(A)
- dendrite
- protein kinase A
- protein kinase C
- hippocampus
- phorbol esters
- cAMP
- action potential
Voltage-dependent K+ channels are the primary regulators of membrane excitability. As a group, they constitute the most diverse of the voltage-gated channels (Rudy, 1988). The large repertoire of K+ channel subtypes available may underlie the distinctive firing patterns expressed by different neurons and by the same cells under different conditions. We have recently found a transient A-type K+ channel to be expressed at high densities in the distal dendrites of CA1 pyramidal neurons (Hoffman et al., 1997). Modulation of these channels could provide the neuron with the means to dynamically and selectively control signal propagation through the dendrites.
The molecular identity of the transient K+ channels recorded in the CA1 hippocampal dendrites is not known for certain, although there is strong evidence in favor of the Shalchannel Kv4.2. Of the two transient K+ channels Kv4.2 and Kv1.4 found in the hippocampus by immunohistochemical techniques, Kv4.2 is primarily located in the soma and dendrites (with the highest degree of immunostaining occurring in dendrites), whereas Kv1.4 is found mainly in axons (Sheng et al., 1992; Maletic-Savatic et al., 1995; Serôdio et al., 1996). Kv4.2 has also been found clustered on the postsynaptic membrane directly apposed to the presynaptic terminal (Alonso and Widmer, 1997). Additionally, both Kv4.2 and the transient K+ channels recorded from CA1 somata are inhibited by arachidonic acid (Villaroel and Schwarz, 1996; Keros and McBain, 1997). Finally, Serôdio et al. (1994)demonstrate that hydrogen peroxide blocks the inactivation of Kv1.4 but not of Kv4.2 channels. Inactivation of the transient channels recorded in CA1 hippocampal neurons is unaffected by externally applied hydrogen peroxide (D. Hoffman, unpublished observations). In our previous report (Hoffman et al., 1997), transient K+ channels in distal dendrites were found to have an activation curve shifted 10–15 mV hyperpolarized compared with those recorded from the soma and proximal (up to 100 μm) dendrites. This result suggested that either a different type of channel is expressed in the two regions or that there is only one channel type, but one that is differentially modulated in the two regions. The immunohistochemical studies that found Kv4.2 located in both the soma and dendrites would support the later conclusion (Sheng et al., 1992; Maletic-Savatic et al., 1995;Serôdio et al., 1996).
Activators of protein kinase A (PKA) and protein kinase C (PKC) have been found to increase the amplitude of EPSPs and population spikes in hippocampal neurons (Malenka et al., 1986; Hu et al., 1987; Storm, 1987; Hvalby et al., 1988; Heginbotham and Dunwiddie, 1991; Slack and Pockett, 1991; Dunwiddie et al., 1992; Pockett et al., 1993). Because the amino acid sequence of Kv4.2 has been shown to contain a potential site for PKA phosphorylation and numerous potential PKC sites (Baldwin et al., 1991; Blair et al., 1991; Anderson et al., 1997), we hypothesized that phosphorylation of transient dendritic K+ channels could potentially account for some of these electrophysiological changes. To test this hypothesis, we made cell-attached patch-clamp recordings of K+ currents from CA1 hippocampal dendrites (180–340 μm from the soma) with and without the inclusion of membrane-permeant activators of both PKA and PKC in the recording pipette. The results suggest that activation of either PKA or PKC can downregulate these channels by shifting the activation curve to more positive potentials. As a test for the functional significance of this downregulation, dendritic action potentials were recorded before and after bath application of PKA and PKC activators. After activation of either kinase, dendritic action potential amplitude was found to increase over 50% in distal dendrites, consistent with a decrease in K+ channel activation.
MATERIALS AND METHODS
Preparation and solutions. Sprague Dawley rats, 5–8 weeks old, were anesthetized with a lethal dose of a combination of ketamine, xylazine, and acepromazine. After they were deeply anesthetized, they were perfused through the heart with cold-modified artificial CSF (ACSF) containing (in mm): 110 CholineCl, 2.5 KCl, 1.2 NaH2PO4, 25 NaHCO3, 0.5 CaCl2, 7.0 MgCl2, 2.4 pyruvate, 1.3 ascorbic acid, and 20 dextrose. After removal of the brain, 400-μm-thick slices were cut using a vibratome, incubated submerged in a holding chamber for 10 min at 34°C, and stored and used for recordings at room temperature.
Hippocampal slices were visualized with a Zeiss Axioskop using infrared video microscopy and differential interference contrast optics. For all recordings, the bath solution contained (in mm): 125 NaCl, 2.5 KCl, 1.25 NaH2PO4, 25 NaHCO3, 2.0 CaCl2, 1.0 MgCl2, and 25 dextrose. In whole-cell experiments, the following were included in the external solution to block synaptic transmission (in μm): 50 d,l-APV (Research Biochemicals, Natick, MA), 20 MK-801 (Research Biochemicals), 10 CNQX (Research Biochemicals), 10 bicuculline (Sigma, St. Louis, MO), and 10 picrotoxin (Sigma). The external solution was bubbled with 95% O2/5% CO2 at ∼22°C, pH ∼7.4. For cell-attached recordings, the normal pipette solution consisted of 125 mm NaCl, 10 mm HEPES, 2.0 mmCaCl2, 1.0 mm MgCl2, 2.5 mm KCl, and 1.0 μm tetrodotoxin (TTX), pH 7.4 with NaOH, to which 100 μm 8-bromo-cAMP (8-br-cAMP; Sigma) was included in certain experiments. For forskolin (Sigma) and phorbol ester (Sigma) recordings, drugs were dissolved in DMSO to 10 mm, kept frozen until use, and then diluted to the appropriate concentration. Whole-cell recording pipettes (10–15 MΩ) were filled with (in mm): 120 KGluconate, 20 KCl, 10 HEPES, 2 MgCl2, 4 Mg-ATP, 0.3 Mg-GTP, and 14 phosphocreatine, pH 7.25 with KOH; pipettes were coated with Sylgard. 1-(5-isoquinolinylsulfonyl)2methyl-piperazine dichloride (300 μm; Sigma) and 8-br-cAMP were dissolved directly into the external bath solution in whole-cell experiments.
Recording techniques and analysis. All neurons exhibited a resting membrane potential between −55 and −73 mV (mean, −66 mV). Cell-attached pipettes (10–20 MΩ) were pulled from borosilicate glass and coated with Sylgard. The tips were visually inspected before use and had uniform tip diameters of ∼1 μm. Channel recordings, using an Axopatch 1D amplifier (Axon Instruments), were analog filtered at 2 kHz and digitally filtered at 1 kHz off-line. Leakage and capacitive currents were digitally subtracted by averaging null traces or scaling traces of similar amplitude. Whole-cell patch-clamp recordings were made using an Axoclamp 2A (Axon Instruments) amplifier in “bridge” mode, low-pass filtered at 3 kHz, and digitized at 10 kHz. Series resistance was 15–40 MΩ. Antidromic action potentials were stimulated by constant current pulses (Neurolog; Digitimer Ltd.) through tungsten electrodes (AM Systems) placed in the alveus.
For activation plots, the chord conductance, as calculated from the peak ensemble current amplitude from a holding potential of approximately −85 mV, was normalized to the maximum value and plotted as a function of the test potential. In the case in which the maximal voltage step did not result in a saturated conductance, conductances were fit to a single Boltzmann, and the peak conductance was used for normalization. For inactivation, the peak ensemble current amplitude for a step to approximately +55 mV was normalized to maximum and plotted as a function of holding potential. Data were binned into either 10 or 20 mV compartments. Curves are nonlinear least-square fits of the data to Boltzmann functions. Inactivation time constants were fit using the Fourier expansion method DISCRETE (Provencher, 1976) and were well fit by a single exponential in most cases. Significance (p < 0.05) was determined by two-samplet tests in all cases except for the PDA effect on action potential amplitude in which a paired t test was used. Error bars represent SEM, and voltages were not corrected for the junction potential (approximately −7 mV).
RESULTS
Isolation of the transient current
Cell-attached patch-clamp recordings from CA1 hippocampal dendrites, in the presence of TTX to block voltage-gated Na+ channels, revealed a large outward current composed of a rapidly inactivating component along with a sustained or slowly inactivating component. Although the transient currentIK(A) was from three to five times the amplitude of the sustained current in the distal dendrites, the transient current was routinely isolated from the sustained current by the voltage protocol shown in Figure 1. In a typical experiment, the patch was held 20 mV hyperpolarized to rest and subsequently depolarized by 20–140 mV in 20 mV increments. Ensemble averages were constructed of 10–30 sweeps per step potential. At the conclusion of the experiment, the membrane was ruptured, and the resting membrane potential was measured, allowing for conversion of the voltage steps relative to rest into absolute voltages. The total outward current recorded for a voltage step from −89 to +51 mV is shown in Figure 1A. A 50 msec prepulse to −29 mV allowed the transient channels to inactivate, leaving only the sustained current (Fig. 1B). The sustained current was subsequently digitally subtracted from the total outward current, resulting in the isolated transient current (Fig. 1C). Occasionally, when a full prepulse ensemble was not obtained, the transient component was taken to be the peak of the total current measured 2 msec into the pulse (before substantial sustained component activation). Activation and inactivation curves constructed using this method were similar to those using prepulses. All channel recordings were made 180–340 μm from the soma.
Modulation of transient K+ channels by activators of PKA
To test for modulation by PKA, we included 100 μm8-br-cAMP, a membrane soluble analog of cAMP, in the patch pipette in 12 dendritic cell-attached recordings. Representative traces (scaled to represent their fraction of maximal conductance) from both control and 8-br-cAMP recordings are shown in Figure2A. In control conditions, a voltage step to −5 mV (near the peak voltage reached during an action potential) activates nearly 50% of the available channels. The inclusion of 8-br-cAMP in the patch pipette reduced this fraction to ∼25%. In the same cell, subsequent bath application of 300 μm H7, a protein kinase inhibitor, increased the fraction back toward control levels. Steady-state activation and inactivation curves were generated from these experiments and are illustrated in Figure 2B. Adding 8-br-cAMP to the patch pipette produced a 13 mV rightward shift in the activation curve, presumably via the activation of PKA (V1/2, −2 and +11 mV for control and 8-br-cAMP, respectively; Fig.2B; Table 1). Similar effects were seen when 50 μm forskolin, an adenylyl cyclase activator, was included in the dendritic patch pipette (V1/2 = +7 mV; n = 5; Table 1). A rightward shift in the activation curve means that at any given potential there will be a decrease in the probability of channel opening. We also found the inactivation curve to be shifted slightly but significantly toward the right (V1/2, −56 vs −50 mV for control and 8-br-cAMP, respectively; Fig. 2B; Table 1). In three of the 12 8-br-cAMP experiments, the kinase inhibitor H7 was bath applied after obtaining a full activation curve. Under these conditions, the activation curve was found to shift progressively back toward control levels in a time-dependent manner (V1/2 = +3.5 mV after 30 min in H7; Fig. 2B; Table 1). Two of the three patches were lost before complete reversal of the 8-br-cAMP effect. On one occasion, however, the patch was held for nearly 1 hr after H7 application. In this patch the curve shifted completely back to control levels (V1/2 = −2 mV; Fig.2B, inset). These results indicate that the shift in the activation curve is attributable to kinase activation and not just a direct effect of 8-br-cAMP on the channel. No significant difference in resting membrane potential was found among groups (Table 1).
Modulation of transient K+ channels by phorbol esters
We investigated the effects of PKC activation on these channels by including one of two different phorbol esters in the patch pipette. Both phorbol diacetate (PDA, 10 μm) and phorbol dibutyrate (PDBu, 10 μm) were found to produce a 15 mV depolarizing shift in the activation curve for transient K+ channels located in the distal dendrites, very similar to that found for PKA activation. Representative traces, scaled to represent their fraction of maximal conductance, from both control and PDA recordings are shown in Figure3A. The inclusion of PDA in the patch pipette led to a 15 mV rightward shift in the activation curve, presumably via the activation of PKC (V1/2, −2 and +13 mV for control and PDA, respectively; Fig. 3B; Table 1). Again, this shift would have the effect of decreasing the probability of channel opening at a given potential. As was the case for PKA activation, there was also a small but significant (6 mV) depolarizing shift in the inactivation curve in the presence of PDA (V1/2, −56 vs −50 mV for control and PDA, respectively; Fig. 3B; Table 1). The steady-state activation curve produced with PDBu in the pipette also was found to be shifted by ∼14 mV (V1/2 = +12 mV; Fig. 3B; Table 1). There was, however, no shift in the activation curve when the inactive phorbol ester 4-α-phorbol was included in the pipette (V1/2 = −2 mV; Fig. 3B; Table 1). These results indicate that the shift in the activation curve is attributable to kinase activation rather than to nonspecific effects of phorbol esters on the channels. Again, no significant difference in resting membrane potential was found among the groups (Table 1).
The voltage dependency of inactivation is altered by 8-br-cAMP and PDA
We have reported previously that the time constant of inactivation of the transient current increases with membrane potential (Hoffman et al., 1997). The same voltage dependency was found in the present study in which the time constant of inactivation for the transient component increased linearly with the amount of depolarization from 11.9 ± 0.9 msec for a step to −5 mV to 27.9 ± 2.3 msec for a step to +55 mV under control conditions (slope = 2.5 msec/10 mV; Fig.4). Inclusion of either 8-br-cAMP or PDA in the patch pipette resulted in a more shallow slope (1.9 msec/10 mV). The time constant at −5 mV was similar to the control value (11.3 ± 0.6 and 10.2 ± 0.9 msec for 8-br-cAMP and PDA, respectively) but was significantly faster than the control value at +55 mV (22.6 ± 2.1 and 22.1 ± 1.6 msec; Fig. 4). Traces from the PDBu group of experiments had time constants of inactivation similar to that of the PDA and 8-br-cAMP groups (slope = 2.0 msec/10 mV), and the inactivation rates in the 4-α-phorbol traces were similar to that of controls (2.5 msec/10 mV; data not shown).
The peak current level from which the time constant was measured is a result of both activation and inactivation kinetics. It seemed possible that this change in slope was the result of incomplete activation under the active kinase conditions. This possibility was ruled out, however, by also measuring the time constant 20 msec into the trace (when activation is presumably complete). The time constants measured in this manner were similar to those measured from the peak current level.
The effects of 8-br-cAMP and PDA on transient channel activation are not additive
In five patches, both 8-br-cAMP and PDA were included the patch pipette. The results, shown in Figure 5, indicate that the effects of the two agents are not additive but rather resemble the shifts seen with either 8-br-cAMP or PDA alone. Representative traces, scaled to represent their fraction of maximal conductance, from both control and PDA with 8-br-cAMP recordings are shown in Figure 5A. The activation curve for 8-br-cAMP plus PDA was shifted to the right by 10 mV compared with that for controls (Fig. 5B; Table 1).
The sustained component is not affected by either 8-br-cAMP or PDA
We also examined the effect of including 8-br-cAMP and PDA in the patch pipette on the sustained component of the total outward current. Ensemble averages of the current remaining at the end of the pulse were used to construct an activation curve for the sustained component. The half-activation values of +2, +7, and +5 mV for control (n = 10), 8-br-cAMP (n = 6), and PDA (n = 8) conditions, respectively, were not significantly different (Fig. 6).
PKA or PKC activation increases the back-propagating action potential amplitude
Dendritic, whole-cell patch recordings of antidromically initiated action potentials were made to assess the functional impact of decreasing the transient K+ channel activity by protein kinase activation. Action potential amplitude, known to decrease with distance from the soma because of an increasing density of A-channels (Turner et al., 1991; Andreasen and Lambert, 1995;Spruston et al., 1995; Hoffman et al., 1997; Magee and Johnston, 1997), was measured before and after bath application of PKA and PKC activators. In distal dendrites, where the amplitude is significantly attenuated by A-channels, both PKA and PKC activation led to a substantial increase in action potential amplitude (Fig.7). Action potential amplitude increased by an average of 78 ± 15% after 10 μm PDA application in distal recordings (Fig.7A,C). In Figure 7A, PKC activation increased action potential amplitude by 62% in a recording 240 μm from the soma. In these experiments, the cell was hyperpolarized to −80 mV to remove residual Na+channel inactivation, which has been shown to be affected by PKC activation (Colbert et al., 1997; Colbert and Johnston, 1998). It has been reported previously that PKC activation does not lead to a significant increase in action potential amplitude in more proximal recordings (Colbert and Johnston, 1998). Similarly, in proximal dendrites, 100 μm 8-br-cAMP had little effect on action potential amplitude in contrast to distal recordings in which the action potential was increased by an average of 51 ± 14% (Fig.7B,C). In Figure 7B, PKA activation increased action potential amplitude by 42% in a recording 280 μm from the soma but had no effect on the action potential recorded 150 μm from the soma. Recordings made at locations in between those shown in Figure 7B resulted in an intermediate but significant increase in action potential amplitude (Fig.7C). Inclusion of H7 in the external solution to oppose kinase activation prevented the effect of 8-br-cAMP on action potential amplitude (Fig. 7C).
The increase in action potential amplitude occurred without a significant increase in the rate of rise. This along with the lack of PKA effect on proximally recorded action potentials indicates that the kinase-dependent increase in amplitude is not caused by an increase in Na+ conductance (Hodgkin and Katz, 1949). This action potential augmentation without an effect on rate of rise was also found after blockade of A-channels by 4-aminopyridine (Hoffman et al., 1997). These data suggest that depolarizing the A-channel activation curve via phosphorylation by PKA or PKC allows dendritic action potentials to propagate farther out into the dendrites than would occur under control conditions.
DISCUSSION
In the present study, we report the downregulation of a voltage-gated K+ channel by activators of two protein kinases, PKA and PKC. Both 8-br-cAMP and forskolin, which activate PKA, shifted the activation curve for dendritic, transient K+ channels by ∼15 mV toward depolarizing potentials. A decrease in transient K+ channel activation in the presence of cAMP activators was also suggested byDeadwyler et al. (1995), although the degree to which activation was decreased was not reported. We also report here that activation of PKC results in a 15 mV shift in the same direction. A recent report has found a PKC effect on Kv4.2 channels expressed in Xenopusoocytes (Nakamura et al., 1997). However, they do not find a shift in the activation curve but, rather, a simple suppression of currents. Although these two findings both result in a decrease in A-current, they are quite different. A shift in the activation curve is a change in the voltage dependence of the probability of channel opening, which indicates an effect on the activation gate of the channel. The decrease in Kv4.2 currents in oocytes, however, was without an effect on the steady-state inactivation curve or the time course of recovery from inactivation, indicating a direct inhibition of the channels by PKC (Nakamura et al., 1997). This difference may mean that transient currents are somehow differentially regulated in the two preparations (perhaps by auxiliary subunits) or that the currents recorded in CA1 dendrites are not the result of Kv4.2 expression. It seems unlikely, however, that Kv4.2 is not at least partially responsible for the dendritic A-currents given the numerous immunohistochemical studies that find Kv4.2 expressed in dendrites, with much less staining of other transient channels (Sheng et al., 1992; Maletic-Savatic et al., 1995; Serôdio et al., 1996). Especially relevant is a recent report showing that both PKA and PKC phosphorylate Kv4.2 (Anderson et al., 1997). Both the C and N terminals of Kv4.2 were shown to be substrates for PKA phosphorylation, and the C terminal is a substrate for PKC phosphorylation.
After PKA or PKC activation, we also report a small but significant depolarizing shift in the inactivation curves. Comparing the inactivation curves for control and 8-br-cAMP conditions in Figure2B, it seems that this shift will have little effect on the channels when the cell is at rest (approximately −65 to −70 mV), with ∼90% of the channels being available for activation. With sustained depolarization, however, there would be a greater percent of channels available for activation with the kinase activated. For example, at −55 mV, only 50% of the channels are available in control conditions compared with 70% with PKA activated. This shift may act to partially compensate for the increased excitability produced by PKA and PKC activation.
It is now well established that back-propagating action potentials in dendrites of CA1 neurons become progressively smaller in amplitude the farther they travel from the soma and may even fail to propagate beyond distal branch points. This decrement in action potential amplitude is found in vivo and in vitro in both the hippocampus and neocortex (Turner et al., 1991; Andreasen and Lambert, 1995; Spruston et al., 1995; Buzsáki et al., 1996; Magee and Johnston, 1997; Svoboda et al., 1997). Although the function of this decrementing action potential is unclear, the high density of transient K+ channels is thought to be primarily responsible for this phenomenon in the hippocampus, because blocking the channels with 4-aminopyridine results in back-propagating action potentials that decrement much less with distance (Hoffman et al., 1997). A decrease in action potential amplitude could also be accomplished by a decreasing density of Na+ channels. By increasing an outward conductance rather than decreasing an inward conductance, however, the cell is able to selectively propagate full amplitude action potentials under certain conditions. Here, we demonstrate one such condition, in which the downregulation of the A-channels by PKA or PKC activation resulted in larger back-propagating action potentials. In a model of a CA1 pyramidal neuron, even a 5 mV shift in the A-channel activation curve was found to significantly increase action potential amplitude in the distal dendrites (M. Migliore, D. A. Hoffman, J. C. Magee, D. Johnston, unpublished observations). If A-channel modulation were to occur selectively in specific regions of the dendritic tree, action potential amplitude may be increased in those regions only, possibly to the extent of preferentially invading one branch over another. Neuromodulatory inputs into the distal dendrites (activating PKA via dopamine, norepinephrine, or serotonin or PKC via muscarinic receptors) may then be able to direct action potentials to specific regions of the dendrite.
It has been reported that the pairing of back-propagating action potentials with EPSPs increases dendritic action potential amplitude and associated Ca2+ influx supralinearly. This pairing was found to facilitate the induction of long-term potentiation (LTP) at CA1 synapses (Magee and Johnston, 1997). We have suggested previously that the mechanism for this EPSP-spike boosting could involve A-channel inactivation (Hoffman et al., 1997). The rapid rate of inactivation of A-channels occurring for small depolarizations such as EPSPs can lead to the amplification of back-propagating action potentials near the site of synaptic input. The present results suggest that downregulation of the A-channels by protein kinase activation, yielding larger dendritic action potentials, might also increase the probability of LTP induction. With high concentrations of 4-AP, which block ∼80% of the total A-channel population, large EPSPs can induce dendritic action potential initiation (Hoffman et al., 1997). It seems unlikely, however, that the 15 mV shift in the activation curve reported here would in itself reduce the A-channel population to the degree necessary for dendritic action potential initiation under normal conditions. If the cell were to undergo a sustained depolarization, such as occurs during bursting or during the tetanus used to elicit LTP, the decreased population of A-channels resulting from kinase activation might increase the likelihood of dendritic action potential initiation.
Given the possible implications of A-channel modulation listed above, persistent downregulation of dendritic, transient K+channels might also contribute to the long-lasting increase in neuronal excitability observed after PKA and PKC activation (Malenka et al., 1986; Hu et al., 1987; Storm, 1987; Hvalby et al., 1988; Heginbotham and Dunwiddie, 1991; Slack and Pockett, 1991; Dunwiddie et al., 1992;Pockett et al., 1993). Many of these effects, including enhancement of EPSPs and increased probability of action potential firing, are similar to those seen in LTP. These observations, along with occlusion experiments and the fact that both PKC and PKA levels increase as a result of the high-frequency stimulation used to induce LTP, strongly suggest that both kinases play important roles in LTP (Malenka et al., 1986; Malinow et al., 1989; Matthies et al., 1991; Wang and Feng, 1992;Klann et al., 1993; Roberson and Sweatt, 1996). Recently, it has been reported that genetic downregulation of PKA results in a decrease in LTP, along with long-term memory deficits (Abel et al., 1997). Also, dopamine acting via the D1/D5 receptor has been shown to increase the magnitude of LTP and to inhibit depotentiation via a cAMP-dependent mechanism (Otmakhova and Lisman, 1996, 1998). The transient K+ channels, as substrates for PKA and PKC, may then play a role in the induction and/or the expression of LTP. An additional association between A-channels and LTP comes from studies involving the mitogen-activated protein kinase (MAPK). Transient K+ channels recorded in CA1 dendrites were found to have their activation curve shifted to the left after blockade of MAPK activation, and Kv4.2 was shown to be phosphorylated by MAPK (Adams et al., 1997) (J. P. Adams, A. E. Anderson, D. A. Hoffman, J. D. English, R. G. Cook, D. Johnston, P. Pfaffinger, J. D. Sweatt, unpublished observations). Other studies show that blocking MAPK activation severely reduces LTP induction in the hippocampus and facilitation inAplysia (English and Sweatt, 1996, 1997; Bailey et al., 1997; Martin et al., 1997).
The downregulation of transient K+ channels in CA1 hippocampal dendrites by activators of PKA and PKC reported here is one of several demonstrations of A-channel modulation. A-type K+ channels are modulated or blocked by neurotransmitters, including serotonin, glutamate, and GABA, by cation concentrations, by auxiliary subunits, by β-amyloid peptide, by arachidonic acid, and by oxidative states (Rudy, 1988; Saint et al., 1990; Chen and Wong, 1991; Wang et al., 1992; Covarrubias et al., 1994;Rettig et al., 1994; Serôdio et al., 1994; Talukder and Harrison, 1995; Good et al., 1996; Keros and McBain, 1997). The vast number and diversity of agents that modulate these channels suggest that they are highly regulated and thus able to finely, dynamically, and selectively control signals as they propagate through the dendrites.
Footnotes
This work was supported by National Institutes of Health Grants NS11535, MH44754, and MH48432, and by Human Frontiers Science Program. We thank Jeff Magee and Rick Gray for comments on this manuscript.
Correspondence should be addressed to Dr. Dan Johnston, Division of Neuroscience, Baylor College of Medicine, One Baylor Plaza, Houston, TX 77030.