Department of Neuroscience, Pennington Biomedical Research Center, Louisiana State University System, Baton Rouge, Louisiana
Submitted 5 November 2004 ; accepted in final form 5 December 2004
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ABSTRACT |
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vagovagal reflex; gastrointestinal motility
The most publicized site of action of CCK is at the level of vagal sensory neurons, where CCK is proposed to act in a paracrine fashion. Such a mechanism of action is supported by a large amount of data indicating that 1) CCK-containing cells are present on the serosal surface of the small intestine; 2) CCK receptors are present on, and transported within, vagal afferents; 3) a large percentage of vagal sensory neurons contain CCK and transcribe CCK-A receptor mRNA; 4) CCK activates intestinal vagal afferent neurons, and this activation is mimicked by intestinal stimuli and attenuated by CCK-A receptor antagonists; and 5) perivagal capsaicin treatment, by destroying sensory C-fibers, significantly attenuates the effects of systemic administration of CCK (2, 3, 12, 18, 31, 33).
However, several lines of evidence indicate that the effects of CCK, especially the satiety effect, might also be mediated via actions at sites other than the peripheral vagal sensory afferents. In fact, systemic administration of the selective CCK-A receptor antagonist devazepide, which crosses the blood-brain barrier, increases food intake in capsaicin-treated, as well as vagotomized, rats (35), and CCK antagonists also attenuate food intake after administration of nutrients that do not increase plasma CCK (7). Furthermore, food intake induces the release of hypothalamic CCK, and microinjections of CCK into the hypothalamus inhibit food intake (4, 13, 41). Similarly, microinjections of CCK into the dorsal vagal complex [DVC; i.e., the nucleus tractus solitarius (NTS) and the dorsal motor nucleus of the vagus (DMV)] inhibit food intake and induce gastric relaxation, and systemic administration of CCK induces c-Fos expression in the DMV and NTS, where CCK receptors have been shown to be present (4, 24, 36, 37).
Electrophysiological analysis of the effects of CCK on DVC cells produced mixed results with respect to the actual effects of CCK as well as the receptor subtypes involved. Plata-Salaman et al. (29) reported that CCK depolarized a large subset of DMV neurons but also hyperpolarized a small fraction of them; both effects were mediated via activation of CCK-A receptors. Conversely, Branchereau et al. (5, 6) reported that application of CCK induced an excitation, an inhibition, or a biphasic excitatory-inhibitory effect on solitary complex neurons. They also concluded that the effects of the sulfated form of CCK octapeptide (CCK8s) were determined by activation of CCK-A and CCK-B receptors; however, their recordings did not distinguish between NTS and DMV neurons.
The aims of the present study, thus, were to investigate and analyze the pharmacological responses of identified gastric-projecting DMV neurons to perfusion with CCK8s.
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MATERIALS AND METHODS |
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Gastrointestinal (GI)-projecting DMV neurons were labeled as described previously (9). Briefly, 10- to 12-day-old Sprague-Dawley rat pups of either gender were anesthetized (indicated by abolition of the foot-pinch withdrawal reflex) with a 3% solution of isoflurane with air (400600 ml/min). To maintain anesthesia, the head of the rat was placed in a custom-made anesthetic chamber through which the isoflurane mixture was perfused. A laparotomy was performed, during which crystals of the retrograde tracer 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate [DiI, DiIC18(3)] were applied to the serosal surface of the stomach fundus, corpus, or antrum/pylorus, and the application site (which covered an 3- to 5-mm2 area along the greater curvature) was embedded in a fast-hardening epoxy resin, which was allowed to dry for several minutes before the entire surgical area was washed with warm saline (9). The wound was closed with 5-0 suture, and the animal was allowed to recover for 1015 days.
Electrophysiology.
The brain stems were removed as described previously (9). Briefly, the rats were anesthetized with halothane; when a deep level of anesthesia was induced, we killed the rats by severing the major blood vessels in the chest. The brain stem was removed and placed in oxygenated Krebs solution at 4°C (see Solution composition). The site of DiI labeling in the stomach was confirmed by visual inspection of the organ. The brain stem was used only from those animals in which the glue covering the site of DiI application was still in place at the time of the experiment. A Vibratome was used to cut six to eight 2- to 300-µm-thick coronal sections containing the DVC, and the sections were stored in oxygenated Krebs solution at 30°C for 1 h before use. A single slice was transferred to a custom-made 500-µl perfusion chamber and kept in place using a nylon mesh. The chamber was maintained at 35 ± 1°C by perfusion with warmed, oxygenated Krebs solution at a rate of 2.53.0 ml/min.
Before electrophysiological recording, GI-projecting DMV neurons were identified using a microscope (model E600-FN, Nikon) equipped with epifluorescent filters suitable for visualizing DiI. Once the identity of a labeled neuron was confirmed, whole cell recordings were made under bright-field illumination using differential interference contrast (Nomarski) optics.
Whole cell recordings were made with patch pipettes (3- to 8-M resistance) filled with a potassium gluconate solution (see Solution composition) using an Axoclamp 2B single-electrode voltage-clamp amplifier (Axon Instruments, Union City, CA). Recordings were made only from neurons unequivocally labeled with DiI. Data were sampled every 100 µs and filtered at 2 kHz, digitized via a Digidata 1200C interface (Axon Instruments), and acquired, stored, and analyzed on an IBM personal computer utilizing pClamp 8 software (Axon Instruments). Recordings were accepted only if the series resistance was <15 M
. In all voltage-clamp experiments, the cells were held at 50 mV. Current-voltage relation curves were constructed by stepping the membrane from 50 to 120 mV in 10-mV increments for 0.51 s. The input resistance was calculated by measuring the instantaneous current displacement obtained by stepping the membrane from 50 to 70 mV. To assess the effects of drugs, each neuron served as its own control (i.e., the results obtained after administration of a drug were compared with those obtained before administration using Student's paired t-test). Cells were classified as responders if CCK8s (30100 nM) induced a current of at least ±20 pA. Values are means ± SE. Significance was set at P < 0.05.
Concentration-response curves were constructed from neurons in which at least three concentrations of CCK8s were tested. At least 5 min were allowed between successive drug applications. Antagonists were applied for 10 min before the agonist was reapplied.
Immunohistochemistry. Rats were injected with fluorogold (20 µg/1 ml saline ip per rat) to label vagal preganglionic neurons innervating the subdiaphragmatic viscera, allowing delineation of the boundaries of the DMV (17, 30, 46).
With the use of a custom-made anesthetic chamber, rats were anesthetized deeply (abolition of foot-pinch withdrawal reflex) with isoflurane, and the abdominal and thoracic areas were shaved and cleaned with 70% ethanol. After an abdominal laparotomy, the stomach was freed from the liver and reflected gently to one side to facilitate access to the gastric wall. Gastric-projecting DMV neurons were retrogradely labeled via microinjections of rhodamine beads (17, 46) or apposition of DiI crystals on the fundus, corpus, or antrum/pylorus (9). As previously described, care was taken to restrict the dyes within the stomach wall and to reduce the possibility of perforating the mucosa. The laparotomy was closed with 5-0 sutures, and the rats were allowed to recover for 515 days to allow retrograde transport of the fluorescent marker to the brain stem. On the day of the experiments, rats were killed with an overdose of halothane and perfused transcardially with 200 ml of chilled saline followed by 200 ml of chilled Zamboni's solution (see Solution composition). In another series of experiments, rats were anesthetized with thiobutabarbital (Inactin, 120 mg/kg ip) and injected with CCK8s (28 µg/kg ip). After 3090 min, the animals were fixed as described above. After extraction, brain stems were immersed in chilled Zamboni's fixative overnight, washed with PBS, and cut into 40-µm-thick coronal sections with a cryostat. The brain stem slices were then mounted on gelatin-coated coverslips and incubated with rabbit anti-CCK-A receptor antibodies (CURE, University of California Los Angeles) diluted 1:200 with 0.1% PBS-BSA for 24 h at 4°C or with rabbit anti-CCK-A phosphorylated receptor diluted 1:250 (R & D Systems, Minneapolis, MN). Sections were then washed in 1% PBS-BSA (3 times over a 2-h period) at room temperature and incubated with secondary goat anti-rabbit antibodies conjugated to Alexa 488 (1:500) for 2 h at 37°C. The brain stem slices were washed in PBS containing 0.1% goat antiserum for 2 h at room temperature before being coverslipped with Fluoromount-G (Southern Biotechnology, Birmingham, AL).
Specimens were examined using a Nikon E400 microscope fitted with epifluorescent filters for tetramethylrhodamine isothiocyanate, FITC, and UV. Cells labeled with rhodamine beads or DiI and/or CCK-A visualized with Alexa 488 were counted on alternate brain stem slices by two independent investigators who were unaware of the treatment. If the cell count differed by >10%, a third investigator analyzed the brain stem slices. The final cell count was the mathematical average of the independent cell counts.
To minimize errors in the counting of DMV somata, we counted only those neurons in which the nucleus was clearly visible. Despite this precaution, we have to consider cell counts as best proportional estimates only, rather than absolute values, when comparing labeled subpopulations. This is of paramount importance, because the surface of the stomach wall covered by application of the retrograde tracers was limited to 35 mm2. Therefore, this provided only a small, but representative, fraction of labeled DMV neurons projecting to the gastric areas of interest.
Sections of brain stem were analyzed from 2 mm caudal to the posterior tip to
3 mm rostral to the anterior tip of the area postrema. Cell count values are means ± SE.
Photographs were taken using a SPOT digital camera (Sterling Heights, MI) mounted on a Nikon E400 fluorescent microscope. Digital images were enhanced using Adobe Photoshop.
Solution composition. Krebs solution contained (in mM) 126 NaCl, 25 NaHCO3, 2.5 KCl, 1.2 MgCl2, 2.4 CaCl2, 1.2 NaH2PO4, and 11 dextrose, with pH maintained at 7.4 by bubbling with 95% O2-5% CO2. Intracellular solution consisted of (in mM) 128 potassium gluconate, 10 KCl, 0.3 CaCl2, 1 MgCl2, 10 HEPES, 1 EGTA, 2 ATP, and 0.25 GTP, with pH adjusted to 7.35 with KOH. PBS consisted of (in mM) 115 NaCl, 75 Na2HPO4·7H2O, 7.5 KH2PO4, and 0.15% Triton X. Zamboni's fixative contained 1.6% (wt/vol) paraformaldehyde, 19 mM KH2PO4, and 100 mM Na2HPO4·7H2O in 240 ml of saturated picric acid and 1,600 ml of H2O, with pH adjusted to 7.4 with HCl.
Statistical analysis.
Values are means ± SE. Intergroup comparisons were analyzed with one-way ANOVA followed by the conservative Bonferroni test for individual post hoc comparisons, Student's paired t-test, or 2 test. Significance was defined as P < 0.05.
Drugs and chemicals. Drugs were made fresh immediately before use and applied to the bath via a series of manually operated valves. Nonsulfated CCK (CCKns) was purchased from Bachem (King of Prussia, PA), DiI from Molecular Probes (Eugene, OR), and fluorogold from Fluorochrome (Denver, CO). Phosphorylated CCK-A receptor antibody was a gift from Dr. A. E. Kalyuzhny (R & D); CCK-A receptor antibody (nonphosphorylated) was a gift from CURE. All other chemicals, including CCK8s, were purchased from Sigma (St. Louis, MO).
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RESULTS |
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CCK8s induced an inward current in subpopulations of DMV neurons. Two minutes of perfusion with CCK8s (30100 nM) induced an inward current in 34% of corpus-projecting neurons (i.e., 30 of 87) and 41% of antrum/pylorus-projecting neurons (i.e., 66 of 159). The remaining 168 (i.e., 64%) neurons, including all the fundus neurons, did not respond to CCK8s. Three more neurons responded to CCK8s with a 50 ± 13 pA outward current. The low occurrence of this type of response to CCK8s prevented us from conducting any type of pharmacological analysis.
Because the response of corpus- and antrum/pylorus-projecting neurons to CCK8s did not differ between the groups, the data obtained from DMV neurons projecting to these two areas were pooled. Furthermore, there was no apparent preferential distribution of cells, whether responsive or unresponsive to CCK8s, along the rostrocaudal extent of the DMV.
The response to perfusion with CCK8s was concentration dependent (30 pM300 nM), the EC50 was 4 nM, the maximum response was reached with 30 nM, and the maximum current amplitude was 42.3 ± 4.7 pA (Fig. 1). Six cells responsive to CCK8s in voltage-clamp configuration were also tested in current-clamp configuration; the spontaneous firing rate was 1.15 ± 0.26 and 2.01 ± 0.26 pulses per second in control and after perfusion with 30 nM CCK8s, respectively (i.e., 104 ± 27% of control, P < 0.05). Twenty-four additional neurons that did not respond to 30 nM CCK8s in the voltage-clamp configuration were also unresponsive to 30 nM CCK8s perfusion when tested in the current-clamp configuration.
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To detect whether the CCK8s-induced current was due to a direct effect of CCK8s on the DMV cell, we compared the amplitude of the CCK8s (30100 nM)-induced inward current in the absence and presence of the synaptic transmission blocker tetrodotoxin (TTX, 0.3 µM). In six neurons, CCK8s induced a 48.0 ± 5.57 pA inward current that recovered to baseline on washout. After 10 min of perfusion with TTX, reapplication of CCK8s in the presence of TTX induced a 37.8 ± 5.71 pA inward current (i.e., 80 ± 9.7% of control, P < 0.05 vs. CCK8s alone; Fig. 3).
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CCK8s-induced inward current is mediated by CCK-A receptors. In 18 DMV neurons, perfusion with 30 nM CCK8s induced a 68.5 ± 5.96 pA inward current. After washout of CCK8s and 10 min of superfusion with the selective CCK-A receptor antagonist lorglumide (0.33 µM), which per se had no effect on the holding current, the CCK8s-induced inward current was significantly attenuated in a concentration-dependent manner (Fig. 5). In contrast, 10 min of pretreatment with the selective CCK-B receptor antagonist triglumide (0.33 µM, n = 12) did not attenuate significantly the CCK8s-induced inward current. Even at the highest concentration tested (3 µM), pretreatment with triglumide did not significantly reduce the CCK8s-induced current (Fig. 5). In six cells in which 3 µM triglumide was first tested against CCK8s, 10 min of perfusion with 1 µM lorglumide and 3 µM triglumide reduced the CCK8s-induced current to the same extent as CCK8s + lorglumide alone (P < 0.05 vs. CCK8s alone, P > 0.05 vs. CCK8s + lorglumide alone; Fig. 5).
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DiI- or rhodamine bead-filled neurons were seen throughout the rostrocaudal extent of the DMV. We counted an average of 40.2 ± 8.16 dye-labeled DMV cells in each animal.
Two different antibodies from CCK-A receptors were tested: the first antibody was raised against the nonphosphorylated receptor and the second against the phosphorylated, i.e., activated (15), receptor. Immunoreactivity to the phosphorylated CCK-A receptor was not observed in four additional rats that did not receive intraperitoneal injection of CCK8s (see MATERIALS AND METHODS), confirming that the antibody was sufficiently specific to recognize the activated, i.e., phosphorylated, form of CCK-A receptor only.
Results obtained from rats pretreated with intraperitoneal injection of CCK8s and tested with the phosphorylated form of the CCK-A receptor or from rats tested with the nonphosphorylated form of the CCK-A receptors were qualitatively and quantitatively similar; thus the data were pooled.
CCK-A receptor immunoreactivity was evenly distributed throughout the rostrocaudal extent of the DMV. The immunoreactivity was restricted to the perinuclear cytoplasm and was not detectable in adjacent processes. CCK-A receptor immunoreactivity colocalized with 65 ± 4.8% of corpus-projecting, 60 ± 3.7% of antrum/pylorus-projecting, and 34 ± 6.8% of fundus-projecting neurons (P < 0.05 vs. corpus and antrum/pylorus; Fig. 6).
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DISCUSSION |
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These data suggest that functional CCK-A, but not CCK-B, receptors are present on subgroups of gastric-projecting DMV neurons. It is possible that these CCK-A receptors are physiologically relevant in the mechanism of action of CCK in the central nervous system (CNS). Given the low circulating concentrations of gut-derived CCK, however, we cannot exclude the possibility that the CCK acting on gastric-projecting DMV neurons is derived from some other source. Thus the full physiological relevance may remain to be established.
Our conclusions are based on the following evidence. Approximately 40% of corpus- and antrum/pylorus-projecting DMV neurons respond to perfusion with CCK8s with an inward current. Conversely, none of the fundus-projecting neurons responded to perfusion with CCK8s. Our data confirm and extend the initial observation by Plata-Salaman and colleagues (29), who showed that 43% of unidentified DMV neurons were depolarized by CCK8s. Contrary to Plata-Salaman and colleagues, who reported that 11% of DMV neurons were hyperpolarized by CCK8s, we observed an outward current (i.e., hyperpolarization) in only 3 of 267 neurons. A possible reason for this discrepancy might be that Plata-Salaman and colleagues recorded from DMV neurons projecting to areas other than those studied in our investigation, which was restricted to gastric-projecting cells. Our data, showing that CCK8s induces an inward current (i.e., an excitatory effect) in gastric-projecting DMV neurons, are in agreement with data showing an excitatory effect of CCK8s in other CNS areas (10, 11, 28, 43).
The CCK8s-induced inward current is attenuated in a concentration-dependent manner by pretreatment with the selective CCK-A receptor antagonist lorglumide. Conversely, the CCK-B-preferring receptor agonist CCK8ns does not induce any current when perfused onto DMV neurons at concentrations as high as 1 µM; a small inward current was induced, however, on administration of 3 µM CCKns, strongly suggesting a nonselective effect. Similarly, pretreatment with the selective CCK-B receptor antagonist triglumide does not attenuate the CCK8s-induced inward current. Furthermore, perfusion with a combination of lorglumide and triglumide attenuates the CCK8s-induced inward current to the same extent as lorglumide alone. Our in vitro data, showing that the effects of CCK8s on DMV neurons are mediated via interaction with CCK-A receptors, are in agreement with biochemical and in vivo results showing that, overall, the satiety and GI effects of CCK8s are mediated via CCK-A receptors (16, 23, 26, 34, 35). Of particular relevance are the data showing that the CCK-mediated effects at the level of the brain stem are mediated via activation of CCK-A receptors (4, 16, 35).
The inward current induced by perfusion with CCK8s is accompanied by a significantly increased input resistance. The reversal potential of the current is close to 90 mV, i.e., close to the reversal potential for potassium, suggesting that the excitatory effects of CCK8s are mediated via closure of a potassium conductance. These results are similar to data reported in other CNS regions, where the excitatory effects of CCK8s were shown to be mediated by closure of potassium conductance (5, 10, 29), although Dun et al. (14) suggested that the effects of CCK in nodose ganglion cells were mediated by an increase in a nonselective cationic conductance.
Our data also show that, after blockade of synaptic transmission with TTX, the response to CCK8s is significantly reduced, suggesting that a portion of the excitatory response to CCK8s is mediated by inputs impinging on DMV neurons, similar to that observed for the parabrachial nucleus and hippocampus (8, 40). Indeed, several authors indicated an excitatory effect of CCK on areas, such as the NTS and area postrema, that have robust projections to DMV and, most importantly, would be preserved in our experimental conditions (1, 46, 16, 36, 38).
Finally, our electrophysiological results are supported by our immunohistochemical data. With the use of two different types of CCK-A receptor antibodies, one recognizing the CCK-A receptor in its phosphorylated state and the other recognizing the nonphosphorylated CCK-A receptor, we observed that CCK-A receptor immunoreactivity is present in a significantly larger proportion of corpus- or antrum/pylorus- than fundus-projecting neurons. CCK-A receptor labeling observed in this study was restricted to cell bodies, as previously reported with autoradiographic and immunochemical methods (19, 24). Interestingly, the phosphorylated CCK-A receptor immunoreactivity was detectable only after intraperitoneal administration of CCK8s, indicating that CCK-A receptors were activated/phosphorylated by circulating CCK8s (15). These data further support the possible role of CCK8s in the central regulation of satiety or gastric functions.
Physiological significance. The CCK-induced gastric relaxation is thought to be one of the mechanisms that mediate the satiety effects of CCK. The DMV comprises the preganglionic parasympathetic neurons that finely modulate gastric tone and motility. Cholinergic neurons in the DMV, in fact, impinge on postganglionic cells that comprise the excitatory cholinergic or the inhibitory nonadrenergic noncholinergic (NANC) pathways that regulate gastric functions (44). CNS-mediated gastric relaxation can thus be obtained via inhibition of DMV neurons that comprise the cholinergic excitatory pathway or via excitation of DMV cells that comprise the inhibitory NANC pathway. Our results, showing that CCK8s has an excitatory effect on DMV neurons, seem to support the hypothesis that the CCK8s-mediated gastric relaxation occurs via an increase in the activity of NANC pathways to the corpus wall, although this mechanism of action is still controversial (42). Under physiological conditions, it is not clear how CCK would reach the brain stem to exert its actions. In fact, the postprandial plasma concentration of CCK is in the low picomolar range, which would not be sufficient to excite DMV neurons. Furthermore, CCK does not readily cross the blood-brain barrier, although portions of the DVC have a "leaky" blood-brain barrier. It is possible, however, that the effects of CCK on DMV neurons are determined by CCK acting as a neurotransmitter or neuromodulator. Indeed, CCK-containing neural projections originating from the NTS or the hypothalamus are present throughout the rostrocaudal extent of the DMV (20).
The hypothesis that the effects of CCK are mediated via activation of an NANC pathway falls short of explaining the lack of effects of CCK8s on fundus-projecting DMV neurons. Because most of the gastric relaxation is mediated by the proximal stomach, which is also the area that supposedly receives most of the NANC innervation, it is possible that the effects of CCK8s are indirect, i.e., mediated by an effect of CCK8s on local inputs impinging on gastric-projecting DMV neurons. Indeed, our data showing that some of the effects of CCK8s are abolished by TTX treatment might indicate this possibility. The lack of CCK8s effects on fundus-projecting neurons might be ascribed to subthreshold (i.e., below resolution) effects on the DMV membrane.
In summary, in the present study, we have shown that CCK-A receptors mediate the excitatory effects of CCK8s on subsets of corpus- and antrum/pylorus-projecting DMV neurons, an action mediated by the closure of a potassium conductance. We have also shown that CCK-A receptor immunoreactivity is present on the membrane of subgroups of gastric-projecting DMV neurons. Taken together, these data would suggest that the CCK8s-mediated gastric relaxation occurs via activation of NANC pathways.
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GRANTS |
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ACKNOWLEDGMENTS |
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Present address of M. W. Lewis: Dept. of Pharmaceutical Sciences, College of Pharmacy and Allied Health Professions, Wayne State University, Detroit, MI 48202.
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FOOTNOTES |
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The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
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REFERENCES |
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