Upper Thoracic Respiratory Interneurons Integrate Noxious Somatic and Visceral Information in Rats

doi:10.1152/jn.00120.2002

Upper Thoracic Respiratory Interneurons Integrate Noxious Somatic and Visceral Information in Rats

Chao Qin, Margaret J. Chandler, Robert D. Foreman, and Jay P. Farber

Department of Physiology, University of Oklahoma Health Sciences Center, Oklahoma City, Oklahoma 73190

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Qin, Chao, Margaret J. Chandler, Robert D. Foreman, and Jay P. Farber. Upper Thoracic Respiratory Interneurons Integrate Noxious Somatic and Visceral Information in Rats. J. Neurophysiol. 88: 2215-2223, 2002. The aim of this study was to determine if thoracic respiratory interneurons (TRINs) might receive peripheral noxious somaticand visceral inputs. Extracellular potentials of 78 respiration-relatedT₃ neurons, whose activity was driven by central respiratory output,were recorded from the intermediate zone in pentobarbital anesthetized,paralyzed, and ventilated male rats. These neurons were identifiedas interneurons by their locations and by the absence of antidromicactivation from the cervical sympathetic trunk and cerebellum.Thoracic esophageal distension (ED) was produced by water inflationof a latex balloon (0.1-0.5 ml, 20 s). A catheter was placed inthe pericardial sac to administer 0.2 ml bradykinin (10⁵ M) for noxious cardiac stimulation. Of 78 TRINs examined forED, activity of 24 TRINs increased and activity of 8 TRINs decreased.Intrapericardial bradykinin increased activity in 26/65 TRINstested and decreased activity in 5 TRINs. Seventy-four TRINs weretested for effects of brush, pressure, and pinch of the chestand upper back areas. No TRINs responded to brushing hair. Low-thresholdresponses to pressure were observed in 27 TRINs. Fourteen TRINswere wide dynamic range and 4 TRINs had high-threshold responses.Peripheral stimuli affected all types of TRINs, including inspiratory,expiratory, and biphasic neurons. Simultaneous phrenic recordingsshowed that effects of various somatic and visceral stimuli onTRINs were independent of central respiratory drive. Various somatovisceraland viscerovisceral patterns of input were observed in TRINs.The results suggested that TRINs participate in intraspinal processingand integration of nociceptive information from somatic fieldsand visceralorgans.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Much effort has been directed at understanding the organization of inputs to spinal interneurons (Edgley 2001; Kirkwood etal. 1987; Lundberg 1979; Zimmermann 1977). For example, spinaldorsal horn interneurons encode noxious and nonnoxious informationand are linked to segmental motor and sympathetic outputs. Theseinterneurons also are subjected to modulatory influences originatingfrom other spinal segments and the brain (Zimmermann 1977). Becausethe majority of inputs to spinal motoneurons originate from intrinsicspinal premotor interneurons, the organization of inputs to differentsubgroups of spinal interneurons is likely to be crucial to outflowsof spinal motoneurons (Edgley 2001).

The respiratory drive from the medulla to the phrenic motoneurons is generally accepted as having a strong monosynaptic component,whereas the intercostal motoneurons are generally viewed as receivingmuch less monosynaptic drive. Thus control of thoracic respiratorymotoneurons is suggested to be dependent mainly on respiratoryinterneurons (Kirkwood 1995; Merrill and Lipski 1987). However,the function of spinal respiratory interneurons probably is notsimply to relay respiratory drive from the medulla. For example,thoracic respiratory interneurons (TRINs) of the cat project tothe contralateral ventral horn and are hypothesized to coordinaterespiratory and/or other motor activities bilaterally (Kirkwoodet al. 1988, 1993; Schmid et al. 1993).

In addition to supraspinal respiration-related inputs, spinal respiratory interneurons at various segments receive other information.Upper cervical inspiratory neurons integrate noxious informationfrom cardiopulmonary and abdominal sympathetic afferents (Yuanet al. 2000) and also are excited by vagal stimulation (Dawkinset al. 1992; Duffin et al. 1994; Lipski et al. 1993). Respiratoryinterneurons within the phrenic motor nucleus respond to stimulationof phrenic afferents (Bellingham and Lipski 1990; Iscoe and Duffin1996). We recently presented evidence that most TRINs receivedpropriospinal inputs from distant (C₁-C₂) spinal segments (Qinet al. 2002b). The aim of this study was to examine responsesof TRINs to various peripheral somatic and visceral stimuli andto determine the incidence of various inputs onto TRINs. A preliminaryreport has been published in abstract form (Farber et al. 2001).

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Experiments were performed on 37 male Sprague-Dawley rats weighing 320-460 g (Charles River, Boston, MA). Anesthesia was initiallyinduced with a bolus injection of pentobarbital sodium (60 mg/kgip) and maintained by supplementary doses (10-15 mg · kg¹ · h¹ intravenous) through a catheter placed in the left jugular vein.The right carotid artery was cannulated to measure arterial bloodpressure. Arterial pressure and pupil diameter were monitoredto determine the anesthesia level during experiments. Followingmuscle paralysis with pancuronium bromide (0.4 mg/kg ip), theanimals were artificially ventilated with room air administeredby a positive-pressure pump (50-60 strokes/min, 3-5 ml strokevolume). Supplemental doses of pancuronium bromide (0.2 mg · kg¹ · h¹ ip) were administered to maintain muscle relaxation throughoutexperiments. Rectal temperature was kept between 37 and 38°C bya servo-controlled heating blanket and overhead infrared lamps.The Institutional Animal Care and Use Committee of the Universityof Oklahoma Health Sciences Center approved the protocols of thisstudy.

The left phrenic nerve crossing the brachial plexus in the neck was exposed, desheathed, and crushed caudally. A bipolar platinumhook electrode was placed around it to monitor central inspiratorydrive. Because continuous infusion of pentobarbital anesthesiaover a long experiment could depress ventilation, an adequatephrenic signal was assured by adding CO₂ ( $<=$ 4%) to the inspiredair. A pair of platinum stimulating electrodes was wrapped aroundthe left cervical sympathetic trunk after it was crushed rostrally.Stimulation parameters were 25-33 V, 1 Hz, 0.2 ms. Bipolar stainlesssteel stimulating electrodes (4-5 mm apart) were placed acrossthe midline of the cerebellum, just below the surface (Edgleyand Grant 1991; Hirai et al. 1988). Stimulation parameters were1-2 mA, 1 Hz, 0.2ms.

Somatic receptive fields of spinal neurons were examined for responses to innocuous brushing with a camel-hair brush, pressurewith a blunt stick, and noxious pinching of skin with a bluntforceps. Neurons were classified as follows: low-threshold (LT)neurons were excited by hair movement and/or pressure; high-threshold(HT) neurons responded only to noxious pinching of the somaticfield; wide dynamic range (WDR) neurons were excited by innocuousstimuli and also had greater responses to noxious pinch of somaticfields. Outlines and descriptions of receptive fields were recordedmanually for all neuronsexamined.

A small latex balloon 1.0 cm in length was attached at the end of PE-240 tubing (ID, 1.67 mm; OD, 2.42 mm) and was insertedperorally into the thoracic esophagus (9-10 cm from the upperfront incisors). Graded esophageal distension (ED) was producedby injecting warm water (0.1, 0.2, 0.3, 0.4, 0.5 ml, 20 s) at0.05-0.1 ml/s (Wei et al. 1997). Esophageal distension (0.3-0.4ml) was used to identify responsive neurons. A high midline thoracotomywas made to expose the pericardial sac by opening the thymus gland.A silicone tubing (0.020 ID, 0.037 OD, 14-16 cm in length) with7-10 small holes in the distal 2 cm was inserted into the pericardialsac over the left ventricle (Euchner-Wamser et al.1994). A solutionof bradykinin (10⁵ M, 0.2 ml) was injected into the pericardial sac for chemicalactivation of afferent endings on the heart. The protocol foradministering bradykinin was to inject warm saline (0.2 ml) intothe pericardial sac and withdraw after 60 s to determine volumeeffects, to inject 0.2 ml of the solution of bradykinin and withdrawafter 60 s, and to rinse the chemicals within the pericardialsac with two to three saline flushes (0.2 mleach).

After the T₃ spinal segment was exposed for extracellular recording, the rat was mounted in a stereotaxic headholder and stabilizedwith vertebral clamps at T₂ and T₅-T₆. Dura mater was carefullyremoved, and the spinal cord was covered with warm agar (3-4%in saline) to improve recording stability. Carbon-filament glassmicroelectrodes were used for recording extracellular potentialsof single T₃ spinal neurons within 0-1.4 mm from the dorsal surfaceand 0.5-2.0 mm lateral to midline in left side of the spinal cord.To identify thoracic respiratory interneurons (TRINs), the followingcriteria were used: 1) respiration-related discharges of spinalneurons were not abolished when the ventilator was stopped for5-10 s. 2) The depth of electrode penetration was limited to 1,400µm so that recorded cells were generally confined to the deepdorsal horn and intermediate zone (Fig. 1). This was assumed toeliminate recording from motor neurons in most instances. 3) Bothpreganglionic sympathetic and spinocerebellar neurons are knownto receive respiratory drive (Edgley and Grant 1991; Gilbey etal. 1982; Hedger and Webber 1976; Hirai et al. 1988). Cells activatedby antidromic stimulation of sympathetic chain or cerebellum wereexcluded from these studies. All neural signals were documentedon-line with the Spike 3 data-acquisition system (CED, Cambridge).An increase or decrease in cell activity >20% of baseline activityduring a stimulus was considered an excitatory or inhibitory response,respectively. Maximal response and duration of response were measuredusing rate histograms (1 s/bin) after various manipulations. Also,inspiratory and expiratory peaks of respiratory phasic activitywere measured using rate histograms (0.1 s/bin) of 10 breathsfor control activity or maximal response to a stimulus. For purposesof illustration, rate histograms with 0.04 s/bin for cell activityare presented in all panels showing expanded recordings. Afterphrenic nerve discharges were filtered and rectified, the signalwas averaged over successive 0.04-s bins. This moving averagewas used to assess any changes in phrenic nerve activity or breathingrate accompanying the various manipulations.

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Fig. 1. Lesion sites of thoracic respiratory interneurons (TRINs) in representative T₃ segment of the rat spinal cord. In all examples,

, TRINs responding to somatic and/or visceral stimuli. $open circle$ , TRINs not responding to various peripheral stimuli. A: inspiratory TRINs. B: expiratory TRINs. C: biphasic TRINs. D: laminae of T₃ segment based on Molander et al. (1989)

. I-X, laminae; CC, column of Clarke; IL, intermediolateral nucleus; IM, intermedial nucleus; Liss, Lissauer's tract; LSN, lateral spinal nucleus; Pyr, pyramidal tract.

After the study of a spinal neuron was completed, an electrolytic lesion (50 µA DC) was made at most recording sites. Thethoracic spinal cord was removed and placed in 10% buffered formalinsolution. Frozen sections (55-60 µm) were examined, and laminaeof lesions were identified (Molander et al. 1989). Statisticalcomparisons were made using Student's paired or unpaired t-testand $chi$ ² analysis. Bonferroni's inequality was used for comparisons betweencontrol conditions and responses to saline and bradykinin. Statisticalsignificance was established as P < 0.05, and data are presentedas means ±SE.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Categories of TRINs

Extracellular recordings from the left side of T₃ spinal segment were made from 78 neurons judged to be TRINs. According tothe timing of increasing firing within the respiratory periodassessed on phrenic nerve activity, TRINs were divided into threedifferent categories: 51 (65%) inspiratory neurons with maximaldischarge during phrenic nerve activity, 15 (19%) expiratory neuronswith maximal discharges during phrenic silence, and 12 (16%) biphasicor phase-spanning neurons that did not fit into the precedingcategories.

Various convergent patterns of TRINs receiving inputs from somatic fields and visceral organs were observed. A comparisonof discharge patterns of TRINs and convergence of inputs are shownin Table 1. Lesions made at recording sites were identified histologicallyfor 38 neurons in the intermediate zone of the spinal cord (Fig.1).

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Table 1. Comparison of discharge patterns of TRINs and their responses to somatic and visceral stimulation

Responses to somatic inputs

Seventy-four TRINs were tested for their responses to various mechanical stimuli of somatic fields. Of these, 45 (61%) TRINsreceived somatic inputs from chest wall, axilla, and upper backarea. Twenty-seven (36%) TRINs were excited by pressure of somaticfields and were classified as LT neurons. Fourteen (19%) WDR neuronswere excited by pressure and had even greater responses to noxiouspinching of somatic fields. Four TRINs were excited only by noxiouspinching and were identified as HT neurons. Examples are presentedin Fig. 2, A-C. No TRIN responded to brushing the hair over thesomatic fields. Comparisons of receptive field properties andrespiration-related firing patterns of responsive TRINs are presentedin Fig. 3A. No expiratory TRIN was classified as a HT neuron.

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Fig. 2. Classification of TRINs to mechanical stimuli of somatic fields. In all examples, traces from top to bottom are integrated phrenic nerve activity (0.04 s/bin), discharges of phrenic nerve, activity of a single thoracic spinal neuron, rate histogram of cell activity (1 s/bin, 0.04 s/bin for panels with extended recordings). A: a TRIN with low-threshold (LT) response to pressure stimulus of somatic field on chest (top). B: a wide dynamic range (WDR) TRIN with response to pressure and greater response to noxious pinch of somatic fields on chest (top). C: a TRIN with high-threshold (HT) response to pinch of axilla (top). A, a-c, B, a-c, and C, a-c: expanded recording of phrenic nerve and cell activity.

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Fig. 3. Comparison of respiratory firing patterns and response of TRINs to somatic and visceral stimuli. A: somatic field properties of TRINs were compared with respiratory firing patterns. B: responses of TRINs to esophageal distension (ED) were compared with respiratory firing patterns. C: responses of TRINs to intrapericardial bradykinin (IB) are compared with respiratory firing patterns. I, inspiratory neuron; E, expiratory neurons; B, biphasic neurons. NR, no response to somatic and visceral stimuli.

Responses to esophageal distension

Esophageal distension (0.4 ml) changed respiration-related activity of 32/78 (41%) TRINs (Table 2). Of these, ED increasedactivity of 24 (31%) TRINs from 13.9 ± 2.3 to 28.8 ± 3.4 imp/smeasured on rate histograms (1 s/bin). An example of a TRIN excitedby ED and a summary for excitatory responses of TRINs to ED areshown in Fig. 4A and Table 2, respectively. Respiratory firingpatterns and excitatory responses of TRINs to ED are comparedin Fig. 3B. For eight TRINs examined for graded ED, stimulus-responsescurves were obtained (Fig. 5A). For TRINs excited by ED, bothinspiratory and expiratory phasic activity significantly increasedwith ED (P < 0.01), whereas phrenic nerve activity did not changeduring ED (Fig. 5B).

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Table 2. Responses of TRINs to esophageal distension (0.4 ml)

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Fig. 4. Responses of TRINs to graded ED. A: a TRIN excited by graded ED. B: a TRIN inhibited by graded ED. A, a-c, and B, a-c: expanded recording of phrenic nerve and cell activity. In all examples, traces from top to bottom are integrated phrenic nerve activity (0.04 s/bin), discharges of phrenic nerve, activity of a single thoracic spinal neuron, rate histogram of cell activity (1 s/bin, 0.04 s/bin for panels with expanded recordings).

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Fig. 5. Summary for effects of ED on respiration-related activity and phasic discharges levels of TRINs. A: stimulus-response relationship of TRINs excited by graded ED. B: summary for excitatory effects of ED (0.4 ml) on phrenic activity and phasic activity of TRINs (n = 24). C: stimulus-response curve of TRINs inhibited by graded ED. D: summary for inhibitory effects of ED (0.4 ml) on phrenic nerve activity and phasic activity of TRINs (n = 8). Excitation and inhibition of TRINs (imp/s) by ED are presented by a maximal change of cell activity during the stimulus, which is calculated by subtracting the mean of 10 s of control activity from the mean of 10 s of the greatest activity during esophageal distension. B/M, breaths per min. PMA, peak moving average of phrenic activity in arbitrary units. *P < 0.05; **P < 0.01.

Spontaneous activity of 8/32 responsive TRINs was reduced by ED (0.4 ml) from 8.0 ± 1.2 to 2.7 ± 1.2 imp/s (1 s/bin, 34% ofcontrol). Table 2 shows the characteristics of TRINs inhibitedby ED. An example of an inhibitory response to ED is shown inFig. 4B. For three TRINs inhibited by graded ED, stimulus-responserelationships are presented in Fig. 5C. Also, ED significantlydecreased inspiratory discharge levels of TRINs independent ofphrenic nerve activity (Fig. 5D).

Responses to intrapericardial bradykinin

Intrapericardial bradykinin (IB) changed the respiration-related activity of 31/65 (48%) TRINs. Respiratory firing patternsof these TRINs and their responses to IB were compared (Fig. 3C).The discharge rate (1 s/bin) of 26/31 (84%) TRINs increased withIB from 13.0 ± 2.1 to 29.6 ± 3.7 imp/s (Table 3), whereas intrapericardialinjection of saline (Fig. 6A) did not change activity of TRINs(13.6 ± 2.2 vs. 13.7 ± 2.3 imp/s). An example of an excitatoryresponse of a TRIN to IB is shown in Fig. 6B, a-c. In contrastto effects of intrapericardial saline on phasic activity of theseTRINs (Fig. 6C), both inspiratory and expiratory phasic activityof TRINs significantly increased with IB (P < 0.01, Fig. 6D),whereas phrenic nerve activity did not change during intrapericardialsaline or IB (Fig. 6, C and D).

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Table 3. Responses of TRINs to intrapericardial bradykinin

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Fig. 6. Excitatory responses of TRINs to IB. A: effect of intrapericardial saline on activity of a TRIN. B: IB increased activity of this TRIN. B, a-c, shows expanded recordings of phrenic nerve and cell activity. C and D: summary for effects of intrapericardial saline or bradykinin on phrenic nerve activity and phasic activity of TRINs (n = 26). **P < 0.01

Intrapericardial bradykinin reduced respiration-related activity of 5/31 TRINs from 10.0 ± 2.6 to 3.6 ± 1.8 imp/s (1 s/bin,36% of control; Table 3), which was compared with effects ofintrapericardial saline (Fig. 7A) on these TRINs (9.7 ± 2.8 vs.9.6 ± 2.7 imp/s). An inhibitory response to IB is shown in Fig.7B, a-c. While overall TRIN discharge decreased, the small samplesize did not show significant effects in each phase of respiration.Furthermore, phrenic activity was unaffected (Fig. 7, C and D).

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Fig. 7. Inhibitory responses of TRINs to IB. A: effect of intrapericardial saline on activity of a TRIN. B: IB decreased activity of this TRIN. B, a-c, shows expanded recording of phrenic nerve and cell activity. C and D: summary for effects of intrapericardial saline or bradykinin on phrenic nerve activity and phasic activity of TRINs (n = 5).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

TRINs are driven by supraspinal respiratory activity (Kirkwood et al. 1988, 1993), and data suggested that they are modulatedby propriospinal inputs from distant segments (Qin et al. 2002b).TRINs might transmit supraspinal respiratory activity to motoneuronsto drive intercostal muscles and are hypothesized to coordinaterespiratory and/or other motor activity bilaterally (Schmid etal. 1993). The present study found that almost two-thirds of TRINswere inspiratory and that 51/78 inspiratory, expiratory, and biphasicTRINs received noxious and nonnoxious inputs from somatic structuresand/or visceral organs. Almost half of TRINs (15/36) respondingto various peripheral stimuli exhibited viscerosomatic or viscerovisceralconvergent patterns. The convergence could have been directlyonto these cells or on presynaptic neurons to these cells. Ineither case, these data support the concept that TRINs participatein intraspinal processing and integration of nociceptive and nonnociceptiveinformation from somatic fields and visceral organs. Effects ofsomatic and visceral inputs on TRINs in the current study aresimilar to results obtained from other studies of spinal interneurons(Edgley 2001; Kirkwood et al. 1987; Lundberg 1979; Zimmermann1977). Kirkwood et al. (1988) noted that respiratory interneuronswere distributed among motor neuron populations as well as moresuperficially. Our search criteria purposely avoided interneuronsthat were deep enough to approximate motor neurons. Our populationstatistics, then, would not reflect these deep cells. Differentelectrode types were used in the present study compared with Kirkwoodet al. (1988) so this also could have influenced cell populationsobtained. Two other points should be considered with respect tothe present classification of interneurons. The first is thatantidromic stimulation of cerebellum and sympathetic chain maynot have always activated spinocerebellar and preganglionic sympatheticcells despite high levels of stimulation. It also is possiblethat there are other presently undocumented ascending cells thatreceive respiratorydrive.

Previous studies showed that application of capsaicin or bradykinin to epicardial receptors in the left and right ventriclein cats elicited increases in respiration (Waldrop 1986; Waldropand Mullins 1987). Also, esophageal distension in dogs reducedinspiratory activation of the diaphragm (Cherniack et al. 1984;DeTroyer and Rousso 1982). In the present study, no significantchanges of respiratory pattern were obtained by monitoring phrenicnerve activity during noxious cardiac or esophageal inputs. Besidespossible species differences, there are two specific issues relatedto our protocol. 1) In the present study, $<=$ 4% CO₂ was added toinspired air to drive respiration in pentobarbital anesthetizedanimals. This could stabilize phrenic nerve activity. 2) An intactvagal afferent pathway typically synchronizes central respiratoryactivity to the ventilator, but we wished to maintain vagal inputsfor cardiac and esophagealstimuli.

Effects of somatic inputs among thoracic neurons

Somatic inputs from muscle proprioceptors (for example muscle spindles) and cutaneous receptors contribute to a multisensorialorganization of spinal interneuron populations (Edgley 2001; Zimmermann1977). Also, afferents from different origins could converge ontocommon interneurons in segmental reflex pathways (Kirkwood etal. 1987). In rats, the majority of upper thoracic spinal neurons(T₂-T₄) within dorsal horn and immediate zone of the spinal cordreceive somatic inputs from skin, muscle, and joints (Hummel etal. 1997). These data are in general similar to findings of thepresent study in which 61% of TRINs responded to various mechanicalstimuli of somatic fields. However, some functional differenceswere revealed by further comparison. First, 23% of T₂-T₄ spinalneurons responded to brushing of the skin (Hummel et al. 1997),whereas none of 78 TRINs had such a response. Second, 41/78 (53%)TRINs responded to pressure on the chest, axilla, and upper back,which were presumed to be proprioreceptive inputs from muscle,joints, and deep tissue. Responses to pressure are more frequentlyencountered in TRINs than in a population of dorsal horn and intermediatezone throacic spinal neurons that were not tested for respiratorymodulation (25%) (Qin et al. 2002a). Third, noxious pinching ofthe skin produced a response in 23% of TRINs, which is much lowerthan 60-74% of T₂-T₄ spinal neurons within dorsal horn and immediatezone that respond to noxious pinch. In particular, only 4/78 (5%)TRINs were identified as HT neurons in the present study, whereas75/224 (33%) spinal neurons were HT (Qin et al. 2002a).

The significance of modulation of TRINs by peripheral cutaneous and muscular inputs is unknown. Previous studies show thatthe respiratory movement pattern or phrenic nerve activity arereflexively changed by cutaneous and muscle afferents, which areprocessed at the spinal level and do not involve supraspinal sites(Decima and Von Euler 1969; Eldridge et al. 1981; Koizumi et al.1961; Remmers 1970). TRINs receiving peripheral proprioreceptiveand noxious somatic inputs could play a role in respiratory proprioreceptivereflexes and spinal processing of noxiousinformation.

Effects of esophageal inputs among thoracic neurons

Spinal dorsal horn and intermediate zone neurons in upper thoracic spinal cord have been electrophysiologically examined forresponses to esophageal distension in cats (Garrison et al. 1992)and in rats (Euchner-Wamser et al. 1993; Qin et al. 2000). Euchner-Wamseret al. (1993) reported that 16% of T₂-T₄ spinal neurons respondedto ED. Of responsive neurons, 84% were excited by ED, 12% wereinhibited, and 4% exhibited a biphasic (excited/inhibited) response.Preliminary results from our laboratory showed that ED excited27% and inhibited 2% of spinal neurons within T₃-T₄ segments ofspinal cord in rats (Qin et al. 2000). In contrast, 41% of TRINsresponded to ED, which was considerably higher than the overallproportion of spinal neurons responding to ED. Response patternsof TRINs were similar to previous studies (Euchner-Wamser et al.1993), i.e., 75% of responsive TRINs were excited and 25% wereinhibited by ED. We also found that ED excited and inhibited bothinspiratory and expiratory phasic activity of TRINs, and no differencewas found between respiratory firing pattern and responses toED. These results suggested that esophageal afferents are a potentiallyimportant input to TRINs and could strongly modulate respiration-relatedactivity of TRINs. It is of interest that some ED-responsive neuronsin T₂-T₄ segments of rats receive convergent inputs from airwaysand respond to various stimuli, such as tracheal distension andhyperinflation as well as smoke and ammonia (Hummel et al. 1997).

Like other viscera, afferent fibers from the esophagus reach the CNS via spinal visceral (sympathetic) afferent fibers tothe spinal cord and via vagal parasympathetic afferent fibersto the nucleus of the solitary tract. In rats, the muscular wallof the whole esophagus consists exclusively of striated musclefiber, which is different from cats, dogs, and humans (Collmanet al. 1992; Khurana and Petras 1991; Neuhuber and Clerc 1990).Spinal visceral afferents from the esophagus are in dorsal rootganglia distributed through the cervical and thoracic spinal cordin rats (Dutsch et al. 1998; Uddman et al. 1995). With respectto parasympathetic innervation, the cervical and upper thoracicportions of the esophagus are innervated predominantly by afferentfibers in the recurrent laryngeal nerves. The lower thoracic andabdominal portions of the esophagus are innervated by vagal afferentfibers originating in the myenteric plexus (Fryscak et al. 1984;Mei 1983; Neuhuber 1987). Because spinal transection at lowercervical segments does not abolish the excitatory responses ofT₃-T₄ spinal neurons to thoracic ED (Qin et al. 2000), it is reasonableto suppose that excitatory effects of ED on TRINs resulted fromactivation of spinal afferents entering the thoracic spinal cord.Because activation of cervical and thoracic vagal afferents reducesresponses of thoracic spinothalamic tract and spinal neurons tonoxious somatic and visceral stimuli (Ammons et al. 1983; Hobbset al. 1989; Thies and Foreman 1983), the inhibitory effects ofED on TRINs observed in the present study might be mediated byvagal-brain stem-spinal pathways. However, spinal visceral afferentpathways cannot be excluded as a cause of inhibitory effects ofesophageal distension onTRINs.

During embryonic development, the esophagus and the lower airways (trachea, bronchi, and lungs) are derived from the samesegment of foregut and share a similar nervous innervation andcontrol (Mansfield 2001). Therefore these organs must coordinatetheir functions through a complex series of reflex and voluntarycontrol. A number of investigations show that esophageal distensionreflexively alters the pattern of ventilation and the distributionof motor activity to the respiratory muscles in humans and animals(Cherniack et al. 1984; Monges et al. 1978; Oliven et al. 1989;Pickering et al. 2002). For example, activation of mechanoreceptorsin the esophagus reflexively inhibits the muscles surroundingthe abdominal cavity and augments the parasternal and expiratorymuscles of the chest wall (Oliven et al. 1989). Physiologically,this reflex reduces the thoracoabdominal pressure gradient duringboth inspiration and expiration and could facilitate the movementof esophageal contents into the stomach. This also may contributeto maintenance of tidal volume and ventilation while eating. Interactionof esophageal afferents and respiratory motor activity also hasbeen suggested as a pathophysiological mechanism of asthma secondaryto gastroesophageal reflux (Harding 2001; Mansfield and Stein1978). The modulation of thoracic respiratory interneurons byesophageal afferents observed in the present study might providea spinal mechanism contributing to the physiological and pathophysiologicalsituations mentioned in the precedingtext.

Effects of cardiac inputs among thoracic neurons

Several groups of projecting and nonprojecting neurons in upper thoracic segments of the spinal cord have been examined electrophysiologicallyfor responses to chemical, electrical or mechanical activationof cardiac afferents in monkeys, cats, and rats (Foreman 1999).In rats, activation of cardiac afferent fibers with noxious intrapericardialchemicals changed background activity in 42% of T₂-T₄ spinal neurons(Euchner-Wamser et al. 1994; Qin et al. 2002a). Of responsivespinal neurons, 85% of neurons were excited, 11% were inhibited,and 4% had excitatory-inhibitory responses. In the present study,intrapericardial bradykinin changed the respiration-related activityin 48% of TRINs. Activity increased in 84% of responsive TRINsand decreased in 16% of TRINs during noxious cardiac stimulation.Furthermore, intrapericardial bradykinin changed both inspiratoryand expiratory phasic activity of TRINs. The similarity of resultsin TRINs and non-respiration-related spinal neurons suggests thatthese different subgroups of spinal neurons process cardiac noxiousinputs in a similarmanner.

The innervation of the heart arises from afferent fibers with cell bodies located in the vagal nodose ganglia and thoracicdorsal root ganglia. Spinal (sympathetic) cardiac afferent fibersenter primarily in the T₂-T₆ spinal segments (Kuo et al. 1984;White 1957). Bradykinin can activate cardiac sympathetic and vagalafferent fibers presumably responsible for producing cardiac painduring myocardial ischemia (Foreman 1999). However, the excitatoryresponses of upper thoracic neurons to intracardiac bradykininare believed to be caused by activation of cardiac sympatheticafferents because vagotomy does not change mean responses (Blairet al. 1984). How afferent inputs to TRINs may influence respiratoryoutput is not understood. However, visceral inputs can affectrespiratory motor activity at the spinal level. For example, electricalstimulation of the sympathetic afferents reflexively producesipsilateral excitation and contralateral inhibition of the triangularissterni (Coon et al. 1995). Furthermore, stimulation of splanchnicafferents can activate phrenic motoneurons and change phrenicnerve discharges and respiratory activity in spinal cats (splanchnic-phrenicreflex) (Albano and Garnier 1983; Decima and Von Euler 1969; Downman1955). Modulation of TRINs by noxious cardiac inputs observedin the present study might provide a spinal mechanism for viscerorespiratoryreflexes; however, the mechanism probably differs from the spinalneural hierarchy for the splanchnic-phrenic reflexes mentionedin the precedingtext.

	ACKNOWLEDGMENTS

The authors thank Dr. C. J. Jou and D. Holston for excellent technicalassistance.

This work was supported by National Institute Neurological Disorders and Stroke Grant NS-35471.

	FOOTNOTES

Address for reprint requests: J. P. Farber, Dept. of Physiology, University of Oklahoma Health Sciences Center, P.O. Box 26901,Oklahoma City, OK 73190 (E-mail address: jay-farber{at}ouhsc.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

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