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The Journal of Neuroscience, March 1, 2001, 21(5):1610-1618
Neural Network Partitioning by NO and cGMP
Nathaniel L. Scholz1, Jan de Vente2, James W. Truman1, and Katherine Graubard1 1 University of Washington, Department of Zoology, Seattle, Washington 98195-1800, and 2 University of Maastricht, Department of Psychiatry and Neuropsychology, 6200 MD Maastricht, The Netherlands
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The stomatogastric ganglion (STG) of the crab Cancer productus contains ~30 neurons arrayed into two different networks (gastric mill and pyloric), each of which produces a distinct motor pattern in vitro. Here we show that the functional division of the STG into these two networks requires intact NO-cGMP signaling. Multiple nitric oxide synthase (NOS)-like proteins are expressed in the stomatogastric nervous system, and NO appears to be released as an orthograde transmitter from descending inputs to the STG. The receptor of NO, a soluble guanylate cyclase (sGC), is expressed in a subset of neurons in both motor networks. When NO diffusion or sGC activation are blocked within the ganglion, the two networks combine into a single conjoint circuit. The gastric mill motor rhythm breaks down, and several gastric neurons pattern switch and begin firing in pyloric time. The functional reorganization of the STG is both rapid and reversible, and the gastric mill motor rhythm is restored when the ganglion is returned to normal saline. Finally, pharmacological manipulations of the NO-cGMP pathway are ineffective when descending modulatory inputs to the STG are blocked. This suggests that the NO-cGMP pathway may interact with other biochemical cascades to partition rhythmic motor output from the ganglion.
Key words: NO; nitric oxide; cGMP; guanylate cyclase; stomatogastric; plasticity; crustacean; central pattern generator; cross talk
INTRODUCTION
Nitric oxide (NO) serves many different functions in the nervous systems of vertebrates (Garthwaite and Boulton, 1995
; Denninger and Marletta, 1999
The rhythmic circuits of the crustacean stomatogastric ganglion (STG) are particularly well suited for studying specific mechanisms of NO-mediated neuromodulation. The STG contains ~30 neurons arrayed into the gastric mill and pyloric motor circuits. These two networks generate very different motor patterns (Heinzel et al., 1993
Parallel modulatory inputs from circulating neurohormones, sensory afferents, and descending projection neurons (Harris-Warrick et al., 1992
Here we show that nitric oxide (NO) is a modulatory neurotransmitter in the STG of the crab Cancer productus. Moreover, we identify a subset of neurons in the gastric mill and pyloric motor networks that express the receptor of NO, an NO-sensitive soluble guanylate cyclase (sGC). These neurons produce cGMP in response to NO. In spontaneously active preparations of the in vitro STG, the two motor patterns collapse into a single conjoint rhythm when the NO-cGMP pathway is blocked. However, NO-mediated signaling is ineffective in the absence of parallel neuromodulatory inputs to the ganglion. Overall, these findings suggest that neural network partitioning in the STG may arise, in part, from interactions between cGMP and other transmitter-evoked biochemical cascades.
MATERIALS AND METHODS
Animals. Adult male rock crabs (Cancer productus) were hand-collected from Puget Sound and maintained without food in seawater aquaria at 12°C. Animals were anesthetized by chilling on ice, and the stomatogastric nervous system (STNS) was dissected as described by Mulloney and Selverston (1974)
Western blotting. Proteins were isolated from gastric mill (GM) muscle (1a and b), brain, and STNS by homogenization in 250 mM Tris-HCl, pH 6.8, 8% SDS, 40% glycerol, 0.01% bromophenol blue, and 20% B-2 mercaptoethanol. After boiling, the homogenates were centrifuged (10,000 × g, 6 min), and the supernatants were frozen at
70°C. Proteins were separated on 8% SDS-PAGE and electrotransferred onto Protran nitrocellulose (Schleicher and Schuell, Keene, NH) overnight at 30 V. Membranes were blocked in 50 mM Tris-HCl, pH 7.8, 150 mM NaCl, 1 mM EDTA, and 0.1% Tween 20 (TBST) containing 5% dried nonfat milk and 5% bovine serum albumin for 2 hr. Membranes were then incubated for 2 hr in rabbit anti-Universal NOS (uNOS; Affinity Bioreagents, Golden, CO) at 1:1000 and mouse anti-actin (Sigma, St. Louis, MO) at 1:500 in TBST and 5% dried nonfat milk. Actin staining was included as a control for loading. After a wash, membranes were incubated with horseradish peroxidase-conjugated donkey anti-mouse (1:1000) and goat anti-rabbit (1:1000) secondary antibodies (both from Jackson ImmunoResearch, West Grove, PA). Detection was enhanced by chemiluminescence (ECL) using a kit from Amersham (Arlington Heights, IL).
Whole-mount immunocytochemistry for uNOS, citrulline, and cGMP. The procedure and controls for uNOS and cGMP immunocytochemistry have been described previously (Scholz et al., 1996
Confocal imaging and analysis. Fluorescently labeled nervous systems (anti-citrulline and anti-cGMP) were imaged with a Bio-Rad (Hercules, CA) MRC 600 laser-scanning confocal microscope as described previously (Scholz et al., 1998
Electrophysiological recordings. Electrophysiological experiments were performed on isolated preparations of the STNS (Fig. 1). The commisural ganglia (CGs), esophageal ganglion (OG), STG, and attached nerves were pinned out on a Sylgard-coated dish and bathed in crab physiological saline (11-13°C). The connections between the anterior ganglia and the STG were intact in all preparations. The STG was desheathed, and a Vaseline well was placed around the ganglion. All pharmacological agents were delivered exclusively to the STG via bath application. For sucrose block experiments, a Vaseline well was used to isolate the anterior ganglia from the STG. The physiological saline surrounding anterior ganglia was then replaced with an isotonic sucrose solution.
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Figure 1. Schematic diagram of the in vitro crab STNS. Anterior is up. avn, Anterior ventricular nerve; CG, commissural ganglion; dgn, dorsal gastric nerve; lgn, lateral gastric nerve; mvn, median ventricular nerve; OG, esophageal ganglion; pdn, pyloric dilator nerve; stn, stomatogastric nerve.
Intracellular recordings from STG neurons were made with an Axoclamp 2A (Axon Instruments, Foster City, CA) using standard techniques (Baldwin and Graubard, 1995
. Motor output from the STG was monitored extracellularly with the use of suction electrodes. Extracellular signals were amplified with a differential amplifier (A-M Systems). Intracellular and extracellular recordings were digitized using a 1401 Plus analog-to-digital converter (Cambridge Electronic Designs, Cambridge, UK) and analyzed using Spike 2 (version 2.01, Cambridge Electronic Designs).
Identification of NO-sensitive STG neurons. Soluble guanylate cyclase (sGC) is a critical component of NO-mediated signaling (Denninger and Marletta, 1999
To identify NO-sensitive neurons in the STG that project anteriorly in the stn, the nerve was cut anterior to the STG and backfilled with neurobiotin (Vector Laboratories, Burlingame, CA). The free end of the stn was placed in a Vaseline well containing neurobiotin (5% in distilled water) for 2 hr at 4°C. The ganglion was then stimulated with SNP-IBMX, processed for cGMP immunocytochemistry, and imaged as described above. Streptavidin Oregon Green 488 (1:200; Molecular Probes, Eugene, OR) was used to visualize the neurobiotin tracer.
Chemicals. SNP, IBMX, and 8-bromoguanosine 3',5'-cyclic monophosphate (8-bromo-cGMP) were obtained from Sigma, and 3-morpholinosydnonimine (SIN-1) was obtained from BIOMOL">Biomol (Plymouth Meeting, PA). 1H-(1,2,4)oxadiazolo(4,3-a)-quinoxalin-1-one (ODQ) was purchased from Alexis (San Diego, CA). ODQ was stored at room temperature as a 100 mM stock in 100% DMSO, and dissolved into crab saline before each experiment (0.1% final DMSO concentration). Control applications of 0.1-1% DMSO alone to the STG had no effect on either cGMP immunocytochemistry or motor pattern production. 2-Phenyl-4,4,5,5-tetramethylimidazoline-1-oxyl-3-oxide (PTIO) was purchased from Calbiochem (La Jolla, CA) and stored as a 10 mM stock in normal crab saline at 4°C. Lucifer Yellow was obtained from Molecular Probes. Unless otherwise noted, solutions were made up fresh at the appropriate time during each experiment. All solutions containing NO donors were used within minutes of dissolution of the donor in crab saline.
RESULTS
Components of the NO-cGMP signaling pathway in the STNS
The STNS is illustrated in Figure 1. To identify NO-synthase (NOS)-like proteins, we probed extracts from crab brain, STNS, and foregut muscle (GM1) with a polyclonal antibody raised against a conserved sequence of NOS (uNOS). It has previously been shown that the crustacean brain contains a biochemically and histochemically identifiable NOS (Johansson and Carlberg, 1994
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Figure 2. NOS expression and activity in the STNS. A, Western blot of proteins extracted from crab muscle, STNS, and brain using a polyclonal antibody raised against a conserved domain of NOS (uNOS). Molecular weights (in kilodaltons) are indicated to the right. B, C, Whole-mount confocal projections of stomatogastric ganglia reacted with a polyclonal antibody raised against citrulline, a byproduct of NOS enzymatic activity. Each projection is a complete image through the ganglion. B, Putative NOS enzymatic activity is present under basal conditions in two projection neurons that enter the STG via the stn (at top; n = 5). Citrulline accumulation is localized exclusively to the posterior stn and the STG (data not shown). C, Citrulline staining in the two input fibers is enhanced when the perineural sheath is removed and the STG is preincubated for 30 min in 1 mM L-arginine (n = 3). Note extensive branching of citrulline-containing terminals in the central synaptic region of the ganglion (neuropil). Because the citrulline antibody cross-reacts with high concentrations of arginine in the nervous system (Eliasson et al., 1997
The uNOS antibody did not reliably stain neuronal structures in whole-mount preparations of the STNS (data not shown). However, in a few preparations (n = 3 of 9 experiments), the antibody labeled a single small somata in the STG. As an alternative approach to localizing NOS, we examined the STG for evidence of NOS enzymatic activity in the form of citrulline production. Citrulline is a byproduct of NO formation from arginine (Bredt and Snyder, 1990
cGMP immunocytochemistry has been used to identify neurons in the STG that contain a NO-sensitive sGC (Scholz et al., 1996
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Figure 3. cGMP immunostaining in the STG. A-C are whole-mount confocal projections of ganglia that have been labeled with a polyclonal antibody raised against cGMP. A, Bath application of NO activates cGMP synthesis in a subset of STG neurons. The in vitro ganglion was treated with an NO donor (10 mM SNP) and processed for cGMP immunocytochemistry (n = 10). As previously reported (Scholz et al., 1996
The presence of citrulline-like immunoreactivity in descending inputs to the STG (Fig. 2B,C) suggests that NO may be released into the synaptic neuropil of the ganglion. To test whether the stimulation of these putative NOS-containing projections could drive cGMP production in the STG to detectable levels, we bathed the ganglion in IBMX and then administered a stimulus to the stn (30 sec at 100 Hz), which elicited a strong excitation of both the gastric mill and pyloric motor rhythms (as monitored with extracellular recordings from the dvn). The STG was then immediately fixed and screened for cGMP immunoreactivity (n = 3). After stimulation, cGMP accumulation was detected within selected processes in the neuropil (Fig. 3C). The appearance of cGMP in the neuropil is consistent with neurons responding to a local release of NO from the descending input fibers.
To determine which STG neurons were NO-sensitive, we identified individual cells (see Materials and Methods) and filled them with Lucifer Yellow. The STG was then exposed to an NO donor and IBMX and processed for cGMP immunocytochemistry (Fig. 4). Overall, 33 STG neurons belonging to eight cell classes were characterized (Table 1). The presence or absence of cGMP immunostaining was consistent, without exception, within each cell class across all experiments. Based on the circuit composition of the congener Cancer borealis (Weimann et al., 1991
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Figure 4. Identification of NO-sensitive and NO-insensitive neurons within the STG. A and B are side-by-side confocal projections (~75 µm total thickness) from the same ganglion. A, NO-induced cGMP immunoreactivity in a subset of ~13 neurons. B, Lucifer Yellow-injected somata from seven identified cells (see Materials and Methods). The colocalization of cGMP and Lucifer Yellow was determined by merging the two projections. Neurons that have nuclei labeled with an asterisk (PD and PY) are NO-sensitive. The remaining cells (DG, VD, and LPG), indicated by squares, are NO-insensitive. The relative position of each asterisk and square is the same for both panels. Note that the VD neuron partially overlaps an unidentified cGMP-containing neuron in the projection. DG, Dorsal gastric; LPG, lateral posterior gastric; PD, pyloric dilator; PY, pyloric; VD, ventricular dilator.
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Table 1. Identification of NO-sensitive neurons in the STG.
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Figure 5. A single NO-sensitive STG neuron projects anteriorly in the stn (top). The stn was backfilled with neurobiotin, and the STG was stimulated with 10 mM SNP and processed for cGMP immunocytochemistry. Anteriorly projecting neurons are labeled green, and NO-sensitive neurons are labeled red. A single cell (yellow) is double-labeled.
Gastric mill motor production requires NO diffusion and sGC activation
We used in vitro preparations of the stomatogastric nervous system to study functional roles for NO-cGMP signaling in the STG. The intact nervous system was pinned out on a Sylgard-coated dish, and a restriction well was constructed to isolate the STG from anterior ganglia (Fig. 6A). In this way, pharmacological agents could be bath-applied exclusively to the STG. The activity of identified STG neurons and the motor output from the ganglion were monitored using intracellular and extracellular recordings.
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Figure 6. The STG generates a gastric mill and pyloric motor pattern in vitro. A, Schematic diagram of the isolated STNS. Anterior is up. Dashed line indicates the placement of a restriction well around the STG. B, Extracellular recordings from three nerves that carry output from the STG reveal distinct gastric mill and pyloric motor rhythms. The top trace shows the firing profiles of two gastric mill neurons (DG, GM), whereas the bottom trace shows the activity of a pyloric neuron (PD). The middle trace shows the VD and IC neurons, which interact with both networks.
The in vitro STG spontaneously generates both a gastric mill and a pyloric motor rhythm (Fig. 6B). The two rhythms are distinct, and they can be distinguished by their periodicity. The gastric mill motor pattern (Fig. 6, top trace) is represented by the neurons that drive the medial tooth subsystem. Bursts of activity in gastric mill neurons (e.g., DG and GM) last for several seconds and have a period of 5-20 sec. By comparison, pyloric-timed activity (PD neurons, bottom trace) is rapid with a period of ~1 sec. In addition, some gastropyloric neurons such as VD and IC (middle trace) are influenced by both networks. Although the STG produces the two rhythms in vitro, only the pyloric motor pattern is generated continuously. The gastric mill pattern is produced episodically and can suddenly stop or start. We used recordings from the medial tooth subsystem to monitor the presence or absence of gastric mill activity. We did not systematically record from the lateral tooth subsystem (LG and MG), and we did not monitor the variants of the gastric mill rhythm that involve the lateral tooth cells (Norris et al., 1994
The accumulation of citrulline within descending inputs to the STG suggests that NO is released within the ganglion under basal conditions when the two networks are conjointly active. Supplementation of the NO-cGMP pathway by bath application of NO donors (1 µM to 1 mM SNP or SIN-1; n = 6) or 8-bromo-cGMP (1 mM; n = 3) had no significant effect on the basic structure of either motor rhythm (data not shown). By contrast, agents that interfere with endogenous NO-cGMP signaling had dramatic effects on both networks. We blocked the extracellular diffusion of NO within the ganglion using bath applications of PTIO, a specific NO scavenger (Akaike et al., 1993
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Figure 7. Pharmacological inhibition of NO diffusion selectively deconstructs the gastric mill motor rhythm. Extracellular recordings of motor output from the STG are shown. Note that the gastric mill rhythm in this preparation is less robust than in the experiment of Figure 6 (i.e., the GM neurons are not firing under basal conditions). Left, Both the gastric mill and the pyloric network are active in normal saline. Middle, Bath application of PTIO (n = 6), an extracellular NO scavenger, selectively shuts down the gastric mill rhythm (the DG neuron falls silent). The pyloric rhythm is excited, GM and VD neurons become active, and all active neurons now fire exclusively in pyloric time. Right, The effect of PTIO is reversible, and the gastric mill motor pattern returns when the STG is returned to normal saline.
We also examined the effects of removing endogenous cGMP production from the system by bathing the ganglion in 50 µM ODQ (n = 12; Fig. 8A), a concentration sufficient to inhibit detectable NO-induced cGMP synthesis (Fig. 3B). The effects of ODQ were identical to those of PTIO, except that the changes in the gastric mill rhythm took place more rapidly (<10 sec). Again, the DG neuron fell silent, and the GM, VD, and IC neurons began firing exclusively in pyloric time. As with PTIO treatments, the GM neurons switched between the gastric mill and pyloric motor networks when sGC activity was blocked (Fig. 8B). Finally, we examined the effect of ODQ on the LG neuron, which drives the protraction of the paired lateral teeth of the gastric mill (Heinzel et al., 1993
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Figure 8. Bath applications of ODQ (n = 12), an inhibitor of NO-sensitive sGC, triggers a rapid and reversible disassembly of the gastric mill motor rhythm. A, As with PTIO (Fig. 7), ODQ inhibits the gastric mill rhythm and excites the pyloric rhythm. B, STG neurons pattern switch when NO-sensitive sGC activity is blocked within the ganglion. Shown are paired intracellular recordings from a GM and PY neuron, and an extracellular recording of the IC and VD neurons (bottom trace). In normal saline (left), the GM neuron fires in gastric time (a single burst in a gastric cycle is shown here), and the PY neuron fires in pyloric time. The IC and VD neurons fire in pyloric time but are inhibited during the GM burst. Within seconds of ODQ application (right), the GM cells pattern switch and begin firing in pyloric time. Note that the IC and VD neurons now participate exclusively in the pyloric motor pattern. Most hyperpolarized membrane potentials: GM,
The modulatory effects of PTIO and ODQ treatments were not limited to neurons that normally participate in the gastric mill network. Both inhibitors also enhanced the pyloric rhythm. For example, ODQ significantly increased the pyloric cycle frequency, from 1.08 ± 0.22 Hz in normal physiological saline to 1.58 ± 0.38 Hz in 50 µM ODQ (p < 0.001; Student's t test; n = 12). An example of the effect of ODQ on pyloric cycle frequency is shown in Figure 8D.
The results from ODQ treatments suggest that ongoing cGMP synthesis is necessary for the normal division of the in vitro STG into two functionally distinct and spontaneously active motor networks. To test whether exogenous applications of cGMP could rescue the effects of ODQ, we pretreated the STG for 10 min with 1 mM 8-bromo-cGMP and then coapplied 1 mM 8-bromo-cGMP and 50 µM ODQ to the STG (n = 5). Surprisingly, ODQ continued to respecify the STG under these conditions (data not shown). Because the main glial sheath that surrounds the dorsal surface of the neuropil was removed in these experiments, stomatogastric neurons were directly exposed to the membrane-permeant analog. Consequently, it is unlikely that 8-bromo-cGMP did not adequately penetrate into the synaptic neuropil. The cGMP analog may be ineffective in this preparation. Alternatively, the NO-cGMP pathway may normally act via cGMP-regulated phosphodiesterases (PDEs), for which 8-bromo-cGMP has a low affinity (Lincoln and Cornwell, 1993
Finally, NO-cGMP signaling appears to be necessary but not sufficient for gastric mill motor production. When descending neuromodulatory inputs to the ganglion are eliminated with a sucrose block to the stn and anterior ganglia, gastric mill-timed motor production ceases, and the pyloric pattern slows down or falls silent. Under these artificially suppressed conditions, bath applications of NO donors (1 µM-1 mM SNP or SIN-1) do not elicit a gastric mill rhythm (n = 5; data not shown). The effects of NO-cGMP signaling are therefore activity-dependent, and they presumably require a coincident release of other neuromodulators within the STG.
DISCUSSION
We have shown that NO-cGMP neuromodulation contributes to the functional separation of the STG into two parallel motor networks. Moreover, under the conditions in which these experiments were conducted (i.e., spontaneous motor production from an in vitro preparation), the signaling pathway is required for the dynamic assembly of the circuit that drives the rhythmic chewing movements of the gastric mill. These results show that NO, acting via sGC, can trigger rapid and reversible shifts in the specification of adult neural circuits (Fig. 9).
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Figure 9. A proposed role for NO-cGMP neuromodulation in the rapid and reversible partitioning of STG motor networks. This model assumes that NO-cGMP signaling interacts with parallel modulatory inputs (data not shown), which are intact and active. Left, Between bouts of feeding, NO-cGMP neuromodulation is absent. The pyloric network is active, and gastric mill units are either silent (open circles) or participate in the pyloric rhythm (filled circle). Middle, When food reaches the gastric mill, NO is released into the STG neuropil from descending inputs or another as yet unidentified source. cGMP accumulates in a subset of neurons, and motor output from the ganglion is partitioned into two parallel rhythms. Previously silent gastric mill neurons become active, whereas others pattern switch from the pyloric network to the gastric mill network (filled circle). Right, NO release stops when food is no longer present in the foregut. cGMP is rapidly hydrolyzed, and the STG returns to a unitary network configuration.
The PTIO data indicate that NO is diffusing within the STG when the pyloric and gastric motor rhythms are both spontaneously active. At least two NOS-like isoforms are expressed in the STNS, and one source of NO is likely to be the pair of descending inputs that terminate in the synaptic neuropil of the ganglion. In this respect, NO is similar to many other anterograde modulatory inputs that have been identified in this system (e.g., Harris-Warrick et al., 1992
The STG neurons that contain a NO-sensitive sGC include the core neurons of the pyloric circuit (PD, PY, and LP) as well as the four GM neurons that can switch between the gastric mill and pyloric networks. An interneuron with an ascending axon (either AB or Int1) is likely to be the last member of the NO-responsive group. Suppression of intrinsic NO-cGMP signaling, using either ODQ or PTIO, speeds up the core pyloric rhythm and causes the GM neurons to pattern switch and burst in pyloric time. Therefore, in the context of the 12 identified sGC-expressing cells, the suppression of the NO pathway results in a ganglion that is dominated by the pyloric motor rhythm. It is important to stress, however, that PTIO- and ODQ-induced changes in firing activity are not limited to neurons that express the receptor of NO. For example, the activity of NO-insensitive neurons (e.g., DG, VD, and IC) also changes when NO-cGMP signaling is inhibited. These indirect effects of NO are likely to reflect synaptic interactions between NO-sensitive and NO-insensitive cells. The nature of these interactions has yet to be determined.
NO donors were not sufficient to activate gastric mill motor output from the STG when descending inputs were blocked. This suggests that NO-cGMP may need to interact with other intracellular signaling pathways that are active in the intact system (Bhalla and Iyengar, 1999
One possible mechanism for interactions between cGMP and parallel biochemical cascades in the STG could involve the activation of cGMP-regulated phosphodiesterases (e.g., PDE3; Delpy et al., 1996
Finally, NO-cGMP signaling is also closely associated with the gastric mill rhythm during STG development. In lobsters, the teeth of the gastric mill and the underlying gastric mill motor pattern first appear at metamorphosis (Casasnovas and Meyrand, 1995
FOOTNOTES Received Sept. 18, 2000; revised Nov. 29, 2000; accepted Dec. 5, 2000.
This work was supported by a National Institutes of Health predoctoral traineeship to N.L.S. and National Institutes of Health Grants NS13079 to J.W.T. and NS15697 to K.G. We thank Jana Labenia for the anti-citrulline staining and technical assistance throughout all phases of this work. We also thank Sarah Gibbs for comments on this manuscript, Wes Grueber for purifying the citrulline antibody, and Ian Kasman for neurobiotin backfills.
Correspondence should be addressed to Dr. Nat Scholz, Environmental Conservation Division, Northwest Fisheries Science Center, 2725 Montlake Boulevard East, Seattle, WA 98112. E-mail: Nathaniel.Scholz{at}noaa.gov.
Dr. Scholz's present address: Northwest Fisheries Science Center, 2725 Montlake Boulevard East, Seattle, WA 98112.
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