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Previous Article | Next Article
The Journal of Neuroscience, January 15, 2003, 23(2):367-372
BRIEF COMMUNICATION
Persistent Changes in Spontaneous Firing of Purkinje Neurons Triggered by the Nitric Oxide Signaling CascadeSpencer L. Smith and Thomas S. Otis Department of Neurobiology and Brain Research Institute, University of California at Los Angeles School of Medicine, Los Angeles, California 90095
ABSTRACT
TOP
ABSTRACT
Introduction
Many types of neurons fire spontaneously because of the activity of pacemaking ion channels. Although endogenous firing can serve as a persistent signal to downstream targets, little attention has been paid to factors that might modulate such intrinsic electrical activity. We tested for modulation of spontaneous firing of Purkinje neurons in cerebellar slices under conditions in which principal synaptic inputs were blocked. Loose-patch recordings from single neurons show that sustained (>40 min) increases in the spontaneous firing rate can be triggered by activation of the nitric oxide-cGMP signaling pathway. Inhibitors of soluble guanylate cyclase and protein kinase G block this modulation. Increases in firing rate are also observed after stimulation of parallel fibers but not in response to basket cell activity. These findings elucidate a novel role for the nitric oxide-cGMP signaling cascade in the brain. This mechanism could permit long-term adjustments in the baseline firing rate of endogenously active neurons in response to changes in afferent activity.
Key words: intrinsic; protein kinase G; cGMP; cerebellum; nitric oxide synthase; pacemaking
Introduction
Spontaneously firing neurons are found in several regions of the brain, including the midbrain, the hypothalamus, the basal ganglia, and the cerebellum (Llinas and Sugimori, 1980
; du Lac and Lisberger, 1995
Cerebellar Purkinje neurons fire with remarkable regularity at high rates even in the absence of excitatory synaptic inputs (Häusser and Clark, 1997
In the cerebellar cortex, elements of the nitric oxide (NO) signaling cascade are expressed at some of the highest levels in the brain. Granule and basket cells express the neuronal form of nitric oxide synthase (NOS) (Bredt et al., 1990
We show in the present study that, independent of fast synaptic transmission, cGMP analogs and NO donors cause a long-term increase in the spontaneous firing rate of Purkinje neurons. Furthermore, the NO-induced increase is blocked by inhibitors of sGC and PKG. We also show evidence that NO generated by parallel fiber activity can cause similar effects. These results highlight an alternative mechanism for circuit plasticity in which nitric oxide signals to groups of spontaneously active neurons to adjust their baseline firing rates.
Materials and Methods
Standard techniques were used to prepare 300-µm-thick parasagittal cerebellar slices (Brasnjo and Otis, 2001
seal resistance) extracellular recordings were made from the soma of visually identified Purkinje neurons in slices from 15- to 22-d-old rats. Glass pipettes (impedance, 1-3 M
Results
To monitor intrinsically generated spontaneous firing, loose-patch extracellular recordings were made from single Purkinje neurons in cerebellar slices continuously bathed in antagonists of GABAA, AMPA, kainate, and (in some cases) NMDA receptors. As reported previously (Häusser and Clark, 1997
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Figure 1. The nitric oxide donor NOR-4 causes an increase in baseline firing rate. A, Example traces taken at times 10 min, 5 min, and 35 min relative to the start of NOR-4 application (C). Calibration: 75 pA, 100 msec. B, Histograms of interspike intervals (ISIs) constructed from 10 min periods at
where A is an amplitude factor, and
is the mean. For the open bars, = 55 msec, SD = 2.9, and A = 0.137; for the filled bars, = 47 msec, SD = 2.7, and A = 0.145. 2 values for both fits are <2 × 10
4. C, Normalized, average firing rate versus time for six neurons. After a 10 min control period, 100 µM NOR-4 was added to the bath as indicated by the bar. On average, firing rates increased 11.4 ± 1.8% (at t = 17 min) and remained elevated for >50 min.
An NO donor causes an increase in spontaneous firing rate
Exposure of slices for 10 min to the nitric oxide donor NOR-4 (100 µM) resulted in a slow increase in spontaneous firing rate that was maintained after removal of the NO donor from the perfusion chamber (Fig. 1). The average increase was to 111.4 ± 1.8% (7 min after NO; n = 6; p = 0.0015) of control, and the relative increase was similar over a wide range of control firing rates (3-50 Hz) (see Fig. 3). Firing rates remained elevated for
50 min after washout of the NO donor (116.8 ± 4.9%, 50 min after NO; n = 6; p = 0.019).
Separate in vitro calibration experiments (see Materials and Methods) indicated that the steady-state concentration of NO achieved under these conditions was ~35 nM. This is five to seven times the NO concentration generated by release from parallel fibers in cerebellar slices as measured by electrochemical methods (Shibuki and Kimura, 1997
cGMP analogs cause an increase in spontaneous firing rate
sGC, the enzyme that synthesizes cGMP and an NO target, is present at high levels in Purkinje neurons; therefore, we tested whether membrane-permeable forms of cGMP increased firing rate. Application of the membrane-permeable cGMP analogs 8p-CPT-cGMP (50 µM) or 8-Br-cGMP (50 µM) for 10 min mimicked the effects of NO donors [8p-CPT-cGMP, 117.7 ± 4.1% 7 min after NO, n = 10, p = 0.0019 (Fig. 2B); 8-Br-cGMP, 118.0 ± 3.1%, n = 4, p = 0.0097]. Similar to NO donors, these increases were long lasting (126.8 ± 8.7% 30 min after 8p-CPT-GMP; n = 10; p = 0.013) (Fig. 2B). As a result of cGMP analog-induced increases in spiking rate, some cells began firing so rapidly that they exhibited a repeating pattern in which the firing rate ramped up to >80 Hz, stopped entirely for several seconds (presumably because of depolarization block), resumed firing at a rate elevated from the control rate, and ramped up until another pause was induced. Such cells were included in the average of cGMP-treated cells in Figure 2B and account for the increase in the variability after drug application. Note also that this hyperexcited firing pattern leads to underestimation of peak firing rates in Figure 2B. To test the idea further that NO activates sGC to increase firing rate, we tested the effects of oxadiazolo quinoxalin-1-one (ODQ), a specific inhibitor of sGC. ODQ alone caused no significant change in firing rate (n = 4). Coapplication of ODQ with NOR-4 blocked the increase in firing rate (Fig. 3C), confirming that sGC activity is required for modulation.
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Figure 2. Membrane-permeant cGMP analogs also increase baseline firing rate. A, Example traces from one neuron in control and 35 min after application of 50 µM 8p-CPT-cGMP. Calibration: 30 pA, 100 msec. B, Average, normalized firing rate versus time for 10 Purkinje neurons. After a 10 min control period, 50 µM 8p-CPT-cGMP was added at the indicated time. On average, the firing rate increased 17.7 ± 4.1%.
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Figure 3. Summary data for 8p-CPT-cGMP, NOR-4, and control cells. A, Plot of the control firing rate for each cell measured over the 5 min period just before drug application versus the firing rate 7 min after the end of the experimental treatment. Each type of experiment is represented by different symbols (control, ; NOR-4,
; 8p-CPT-cGMP,
; 8-Br-cGMP,
), and the error bars indicate SD. The diagonal dotted line indicates no change in firing rate. The vertical distance between the marker and the dotted line represents the number of additional spikes every second. * denotes the example cell in Figure 1, and # indicates the example cell in Figure 2. Inset, Shown at a compressed scale to show the cells with higher firing rates. B, Average time course of four control cells. Although there is a small tendency toward increased firing rates, it is not significant and does not resemble the increases seen in the experimental conditions. C, Histogram shows average change in firing rate at t = 5-10 min after drug application compared with control (
PKG is necessary for NO-induced increase in firing rate
A rise in cytoplasmic cGMP concentration in Purkinje cells could increase endogenous firing through at least two types of mechanisms. Cyclic nucleotide-gated (CNG) cation channels could increase spiking by depolarizing the membrane potential. Alternatively, cGMP could activate PKG, a protein kinase expressed at high levels by Purkinje neurons (Lohmann et al., 1981
Testing for endogenous activity-dependent production of NO
Because NOS is expressed by both granule neurons and basket cells, we tested whether activity in these neurons was able to generate NOS-dependent increases in firing rate. To stimulate PFs, the axons of granule neurons, we used previously published stimulation parameters to ensure that substantial NO release occurred (Shibuki and Kimura, 1997
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Figure 4. Stimulation of parallel fibers or basket cells to generate endogenous NO. A, To maximize NO production from PFs, presynaptic fiber volleys were measured and stimulus intensity was adjusted before each experiment. Average fiber volley across all experiments was 3.0 ± 1.4 mV (range, 2-5 mV). Calibration: 3 mV, 0.5 msec. B, An example of one experiment. Five trains of stimuli (20 Hz for 5 sec, 6 sec intertrain interval) was delivered to the PFs at t = 0 min. C, Average results from seven control cells; D, eight NOS inhibitor cells. NOS inhibitors block an increase in firing rate. At t = 20 min, control cells tend toward higher firing rates, whereas cells in the presence of NOS inhibitors tend toward baseline firing rates. E, Paired recordings (1 whole-cell recording from a basket cell, 1 extracellular recording from a synaptically connected Purkinje neuron) were established in the absence of picrotoxin. Calibration: 20 mV, 75 pA, 100 msec. F, After addition of 100 µM picrotoxin to block the fast synaptic inhibition, a presynaptic basket cell was stimulated at time t = 0 min. Little change in firing is visible in this example recording from the connected Purkinje neuron. G, On average, no significant increase could be detected in four pairs.
We next tested whether basket cells could be stimulated to produce NO and cause increases in Purkinje neuron firing rates. A whole-cell recording was established from a basket cell, and an extracellular recording was used to identify a Purkinje neuron inhibited by that basket cell. An example of such a pair is shown in Figure 4E. After a connected pair had been identified in picrotoxin-free solution, GABAA receptors were blocked by adding picrotoxin to the bath. The basket cell was then prevented from firing by injection of hyperpolarizing current while a baseline firing rate was measured in the Purkinje neuron. After baseline data had been collected, the basket cell was made to fire bursts of action potentials by repeated depolarizing and hyperpolarizing current injections. Results from an example recording are shown in Figure 4F, and average results from four connected pairs are shown in Figure 4G. These manipulations had no significant effect on the firing rate of Purkinje neurons (Fig. 4G) (101.2 ± 1.8%; n = 4; p = 0.55), and therefore the effects of NOS inhibitors were not tested.
Discussion
These experiments show that brief exposure to NO donors or cGMP can trigger long-lasting increases in the spontaneous firing rate of Purkinje neurons in the absence of fast synaptic inputs. Stimulation of PFs using a protocol known to release NO also caused increases in Purkinje neuron firing rates that were blocked by NOS inhibitors. Together, the data provide strong evidence that the observed effect is a result of NO stimulating sGC to generate an increase in cGMP concentration. cGMP could affect several different targets, including CNG channels, phosphodiesterases, or PKG (Hofmann et al., 2000
This modulation caused relative increases in firing rate up to 25%. Although this may seem moderate, given baseline firing rates from 15 to 60 spikes/sec, this represents 4-15 extra spikes every second. Changes of this magnitude will most likely make a strong contribution to the output of the cerebellar cortex.
Previous work has suggested that NO modulates neural activity by changing excitatory synaptic strength. However, these studies indicating a role for NO in hippocampal long-term potentiation (Schuman and Madison, 1991
To change the spontaneous firing rate of a neuron, ionic conductances in the cell membrane must be altered. At least two channels are attractive candidates: large-conductance, Ca2+-activated K+ channels (BK) and the channels responsible for persistent or resurgent Na+ current. In smooth muscle tissue, BK channels are facilitated by NO-cGMP (Archer et al., 1994
A second candidate conductance is a class of TTX-sensitive Na+ currents that generates inward current flow between spikes (Uteshev et al., 1995
Our results suggest that integrated, local activity triggers long-term increases in Purkinje neuron excitability, but which afferents trigger NO production? We investigated two possible sources of endogenous NO production. Cerebellar granule cells and basket cells express NOS at high levels (Bredt et al., 1990
A major component of the output of cerebellar cortex consists of pauses in persistent firing of Purkinje neurons. These pauses facilitate firing of target premotor neurons in the cerebellar nuclei and vestibular nucleus (Eccles et al., 1967
Given that NO-cGMP elements are expressed throughout the brain, this mechanism may be widespread, producing activity-dependent, persistent adjustments in the baseline firing rate of endogenously active neurons.
FOOTNOTES Received Sept. 16, 2002; revised Oct. 17, 2002; accepted Oct. 22, 2002.
This project was supported by a grant from the Whitehall Foundation (T.S.O.) and National Science Foundation Training Grant DGE-997802 (S.L.S.). We are grateful to G. Brasnjo, J. Dzubay, J. Feldman, L. Ignarro, P. Meera, and F. Schweizer for comments on this manuscript and A. Jacobs for assistance with the nitric oxide measurements.
Correspondence should be addressed to Thomas S. Otis, Department of Neurobiology and Brain Research Institute, University of California at Los Angeles School of Medicine, 650 Charles Young Drive South, Los Angeles, CA 90095. E-mail: otist{at}ucla.edu.
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