Interleukin-1beta  alters brown adipose tissue but not renal sympathetic nerve responses to hypothermia

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Interleukin-1 $beta$ alters brown adipose tissue but not renal sympathetic nerve responses to hypothermia

Michael J. Kenney, Frank Blecha, Donald A. Morgan, and Richard J. Fels

Department of Anatomy and Physiology, Kansas State University, Manhattan, Kansas 66506; and Department of Internal Medicine, Cardiovascular Center, University of Iowa College of Medicine, Iowa City, Iowa 52242

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Proinflammatory cytokines and acute physical stress influence sympathetic nerve discharge (SND). Because interleukin-1 $beta$ (IL-1 $beta$ )produces physiological responses that require central neural integrationand because the sympathetic nervous system mediates physiologicalresponses to environmental stress, we hypothesized that IL-1 $beta$ modulates SND responses to acute physical stress. Therefore, thisstudy examined the effects of IL-1 $beta$ (290 ng/kg iv) and mild hypothermiaon renal and interscapular brown adipose tissue (IBAT) SND regulationin chloralose-anesthetized rats. IBAT SND did not change afterIL-1 $beta$ administration but was significantly increased during acutemild hypothermia, which was induced 60 min after IL-1 $beta$ treatment.Renal SND was unchanged after IL-1 $beta$ administration and duringhypothermia. Acute hypothermia, without prior IL-1 $beta$ administration,did not alter IBAT and renal SND. Increases in IBAT SND duringsustained (120 min) hypothermia were significantly higher in IL-1 $beta$ -treatedrats compared with saline-treated rats, whereas renal SND responsesto sustained hypothermia did not differ among groups. Exposureto acute cold stress after sustained hypothermia produced greaterincreases in IBAT SND in IL-1 $beta$ -treated rats compared with saline-treatedcontrols. These data suggest that IL-1 $beta$ alters IBAT SND responsesto acute and sustainedhypothermia.

sympathetic nerve activity; cytokines; chloralose; Sprague-Dawley rats

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

INCREASING EVIDENCE from the disciplines of neuroscience and immunology indicate that cytokines can engage the nervous system.For example, intravenous and intraportal administration of interleukin-1 $beta$ (IL-1 $beta$ ) in anesthetized rats increases afferent vagal nerve activity(3, 22), intravenous and intracerebroventricular administrationof IL-1 $beta$ alters efferent sympathetic nerve discharge (SND) (15,16, 23, 28, 32), and plantar injection of IL-1 $beta$ inducestransient spontaneous discharges in primary afferent fiber filaments(12). Important relative to the current study, IL-1 $beta$ sensitizessomatic sensory nerve endings to mechanical and thermal stimulation(12) and sensitizes visceral afferents to ischemia and histamine(11).

Changing the level of activity in peripheral sympathetic nerves in response to external and internal stimuli is an importantway that mammals maintain physiological homeostasis. Importantly,SND responses to a given stimulus can be substantially modulatedwhen a second stimulus is combined with the first. For example,muscle SND responses evoked by rhythmic exercise are potentiatedby isocapnic hypoxia (29), hypertonic but not normal salineinfusion produces renal sympathoexcitation after hemorrhage inanesthetized rabbits (30), and elevated cerebrospinal fluidosmolality produces vasoconstriction of the skin in rabbits exposedto heat (34).

Does IL-1 $beta$ modulate SND responses to acute physical stress? Because IL-1 $beta$ enhances the responsiveness of primary afferentsto various experimental paradigms (including mechanical and thermalstimuli) (11, 12) and because sympathetic neural circuitsare affected by alterations in the physiological status of theanimal (17), we reasoned that IL-1 $beta$ might play a neuromodulatoryrole in sympathetic regulation to acute environmental stress.The aim of this study was to test the hypothesis that IL-1 $beta$ altersinterscapular brown adipose tissue (IBAT) and renal SND responsesto mild hypothermia in chloralose-anesthetized rats. IBAT nerverecordings were completed because activation of this nerve enhancesheat production through nonshivering thermogenesis (8-10, 14,19). Renal nerve recordings were completed because hypothermiareduces the level of renal SND (17) and because the sympatheticinnervation to the kidney influences renal blood flow, renin release,and salt and water retention by the renal tubules (2), responsesthat are part of the integrative physiological changes associatedwith hypothermia and sicknessbehavior.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

General procedures. The surgical procedures and experimental protocols used in the current study were approved by the Institutional Animal Careand Use Committee. Male Sprague-Dawley rats (345 ± 2 g) were initiallyanesthetized with methohexital sodium (Brevital, 50-60 mg/kg ip)(17, 18, 28). Catheters were placed in the femoral veinfor administration of $alpha$ -chloralose (initial dose of 50 mg/kg andmaintenance doses of 35-45 mg · kg¹ · h¹) (17, 18, 28), maintenance doses of methohexital sodium(10-20 mg/kg during surgical interventions) (17, 18, 28),and IL-1 $beta$ or saline. The rats were intubated, paralyzed with gallaminetriethiodide (initial dose of 5-10 mg/kg iv and maintenance dosesof 10-15 mg · kg¹ · h¹) (17, 18), and artificially ventilated. Femoral arterialpressure and heart rate (HR) were recorded using standard procedures.Colonic temperature (T_c) was measured with a thermistor probeinserted ~5 cm into the colon and was kept at 38°C during surgicalinterventions by a heating plate located beneath the animal andby a heatlamp.

Neural recordings. Activity was recorded biphasically with a platinum bipolar electrode after capacity-coupled preamplification (band pass, 30-3,000Hz) from the central end of cut renal and IBAT sympathetic nerves.The renal nerve was isolated retroperitoneally (17, 18, 28),and the IBAT nerve was isolated after visualization of the IBATafter a nape incision (13). The nerve-electrode preparationswere covered with a silicone gel. The sympathetic nerve potentialswere full-wave rectified and integrated (time constant, 10 ms),which produced a smooth tracing of the synchronized discharges(28). The level of activity in sympathetic nerves was quantifiedafter integration as volts × seconds and corrected for backgroundnoise after ganglionic blockade (15 mg/kg trimethaphan camsylate)or nerve crush (17, 18, 28).

Experimental protocols. Mean arterial pressure (MAP), HR, and SND (IBAT and renal) were continuously recorded during four experimental protocols,three of which included the intravenous administration of IL-1 $beta$ (290 ng/kg). IL-1 $beta$ was dissolved in phosphate-buffered saline,and rats that received this cytokine were administered a singledose. Protocol I determined the combined effect of IL-1 $beta$ and acutecold stress that produced mild hypothermia on renal and IBAT SND(n = 8). IBAT and renal SND were recorded before (control) andfor 60 min after IL-1 $beta$ administration (T_c maintained at 38°C duringthese periods). Sixty minutes after IL-1 $beta$ , T_c was decreased from38 to 36.1 ± 0.3°C (time to reduce T_c, 11 ± 2 min) by turningoff the heat sources and placing packaged ice on the metal heatingplate in close proximity to the animal. As the target T_c was neared,the ice was removed from the table, allowing T_c to reach a steadystate so that SND measurements could be completed. IL-1 $beta$ was administered60 min before initiation of acute cold stress because in chloralose-anesthetizedrats IL-1 $beta$ produces progressive (peak increases 45-60 min afterIL-1 $beta$ ) and significant increases in splenic and lumbar SND butdoes not change the level of renal and IBAT SND (28). Therefore,although it was expected that IL-1 $beta$ alone would not change thelevel of IBAT and renal SND, we waited an extended period of timeafter IL-1 $beta$ administration before inducing hypothermia to allowtime for this cytokine to interact with central neural circuits.Protocol II determined the effect of mild hypothermia (no priorIL-1 $beta$ administration) on renal and IBAT SND (n = 17). A 60-mincontrol period was completed (300 µl iv saline, administered atthe beginning of this period) before T_c was decreased from 38to 36.0 ± 0.1°C (time to reduce T_c, 11 ± 1 min) using the samecooling protocol as described above. After the level of SND at36°C was measured, the cold stimulus was maintained in five experimentsuntil T_c reached 31°C. Protocol III determined the effect of IL-1 $beta$ administration without subsequent hypothermia (T_c maintained at38°C) on IBAT and renal SND (n = 5). SND recordings were maintainedfor 75 min after IL-1 $beta$ to control for the time required to completeprotocol I. Protocol IV also examined the combined effect of IL-1 $beta$ and mild hypothermia on IBAT and renal SND; however, the sequenceof interventions was different than that in protocol I. IL-1 $beta$ (n = 8) or saline (n = 8) was administered 5 min before T_c wasdecreased from 38 to 35.5°C (time to reduce T_c, 10-15 min; samecooling protocol as described above). T_c was maintained at thislevel for 120 min (sustained hypothermia). At this time, T_c wasreduced an additional 0.5°C from 35.5 to 35°C. A brief summaryof the experimental protocols is shown in Table 1.

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Table 1. Summary of experimental protocols

Data and statistical analysis. Values are means ± SE. Control values of SND were taken as 100%. Results were analyzed using analysis of variance techniqueswith a repeated measures design followed by Bonferroni post hoctests. P < 0.05 indicated statisticalsignificance.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Protocol I: effect of IL-1 $beta$ and acute hypothermia on IBAT and renal SND. Figure 1A shows traces from a representative experiment of simultaneously recorded renal and IBAT SND bursts during control(T_c = 38°C; left), 60 min after IL-1 $beta$ administration (T_c = 38°C;middle), and after application of acute cold stress, which wasinitiated 60 min after IL-1 $beta$ and produced mild hypothermia (T_c= 36.5°C; right). In contrast with the renal nerve, there waslittle spontaneous IBAT nerve activity during control. Renal andIBAT SND were unchanged from control 60 min after IL-1 $beta$ . However,IBAT SND was markedly increased, whereas renal SND remained unchanged,when T_c was reduced to 36.5°C. Mean data for the group (n = 8)are presented in Fig. 1B. IBAT SND remained unchanged 60 min afterIL-1 $beta$ (T_c = 38°C) but was significantly increased 460 ± 144% fromcontrol after acute cold stress, which was initiated 60 min afterIL-1 $beta$ and produced mild hypothermia (T_c from 38 to 36.1 ± 0.3°Cin 11 ± 2 min). Renal SND was not significantly changed afterIL-1 $beta$ ( $-$ 8 ± 9%) or during hypothermia ( $-$ 25 ± 10%). MAP (control,110 ± 4 mmHg; IL-1 $beta$ , 100 ± 7 mmHg; hypothermia, 98 ± 7 mmHg) andHR (control, 345 ± 15 beats/min; IL-1 $beta$ , 336 ± 8 beats/min; hypothermia,318 ± 12 beats/min) were not significantly changed after IL-1 $beta$ or hypothermia.

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Fig. 1. A: traces of integrated renal sympathetic nerve discharge (SND) and interscapular brown adipose tissue (IBAT) bursts recorded before (control; left), 60 min after interleukin-1 $beta$ (IL-1 $beta$ ) administration (right), and after acute cold stress (right), which was initiated 60 min after IL-1 $beta$ and produced mild hypothermia [colonic temperature (T_c) = 36.5°C]. B: average IBAT and renal SND responses 60 min after IL-1 $beta$ administration and after acute cold stress, which produced mild hypothermia (T_c = 36.1 ± 0.3°C). SND is expressed as a percentage of control activity. *Significantly different from control.

Protocol II: effect of acute hypothermia on IBAT and renal SND. The effect of acute cold stress, which produced mild hypothermia (T_c from 38°C to 36 ± 0.1°C in 11 ± 1 min) without prioradministration of IL-1 $beta$ on the level of IBAT and renal SND, wasdetermined in 17 experiments. IBAT (+36 ± 29%) and renal ( $-$ 5 ±5%) SND did not change from control during hypothermia. MAP (control,118 ± 4 mmHg; hypothermia, 108 ± 4 mmHg) and HR (control, 370± 8 beats/min; hypothermia, 350 ± 9 beats/min) were significantlyreduced during hypothermia. IBAT SND was increased 341 ± 47% (P< 0.05) and renal SND was decreased 27 ± 8% (P < 0.05) in fiveexperiments in which T_c was reduced to 31°C.

Protocol III: effect of IL-1 $beta$ on IBAT and renal SND. The effect of IL-1 $beta$ without subsequent hypothermia on IBAT and renal SND was determined in five experiments. IBAT SND ( $-$ 14± 10%) was unchanged, whereas renal SND was reduced ( $-$ 22 ± 9%,P < 0.05), from control 75 min after IL-1 $beta$ . MAP (control, 108± 5 mmHg; IL-1 $beta$ , 110 ± 6 mmHg) and HR (control, 395 ± 12 beats/min,IL-1 $beta$ , 398 ± 13 beats/min) were unchanged from control levelsafter IL-1 $beta$ .

Protocol IV: effect of IL-1 $beta$ and acute and sustained hypothermia on IBAT and renal SND. Figure 2 summarizes IBAT (A) and renal (B) SND responses to IL-1 $beta$ (n = 8) and saline (n = 8) administration at the followingexperimental points: acute hypothermia (T_c = 35.5°C) producedby cold stress, which was initiated 5 min after IL-1 $beta$ and salineadministration; at 60 and 120 min of sustained mild hypothermia(T_c = 35.5°C); and after a second period of cold stress, whichreduced T_c from 35.5 to 35°C. Reducing T_c from 38 to 35.5°C immediatelyafter IL-1 $beta$ or saline administration did not affect IBAT SND.Increases in IBAT SND at 60 and 120 min of sustained hypothermiawere significantly higher in IL-1 $beta$ -treated rats than in saline-treatedrats. Reducing T_c from 35.5 to 35°C after sustained hypothermiaincreased (P < 0.05) IBAT SND from levels recorded at 35.5°C inboth IL-1 $beta$ - and saline-treated rats; however, increases in IBATSND were significantly higher in rats that received IL-1 $beta$ . RenalSND was significantly reduced from control during each experimentalintervention in rats pretreated with IL-1 $beta$ and saline; however,responses did not differ among groups. MAP (IL-1 $beta$ : control, 136± 4 mmHg; sustained hypothermia, 113 ± 7 mmHg; saline: control,124 ± 10 mmHg; sustained hypothermia, 98 ± 7 mmHg) and HR (IL-1 $beta$ :control, 385 ± 12 beats/min; sustained hypothermia, 312 ± 16 beats/min;saline: control, 368 ± 13 beats/min; sustained hypothermia, 285± 7 beats/min) were significantly reduced from control duringsustained hypothermia (at 60 and 120 min, only 60-min data included)in IL-1 $beta$ - and saline-treated rats.

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Fig. 2. Average IBAT (A) and renal (B) SND responses to IL-1 $beta$ and saline administration at the following experimental points: after an initial bout of cold stress, which produced acute hypothermia (T_c = 35.5°C); at 60 and 120 min of sustained hypothermia, with T_c maintained at 35.5°C; and after a second bout of cold stress, which reduced T_c from 35.5 to 35.0°C. SND is expressed as a percentage of control activity. *Significantly different from levels of IBAT SND recorded at 35.5°C (120 min). $dagger$ Significantly different from levels of IBAT SND recorded in saline-treated rats.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

This study examined the effects of IL-1 $beta$ and mild hypothermia on renal and IBAT SND regulation in $alpha$ -chloralose-anesthetizedrats. The following observations were made: First, induction ofacute mild hypothermia (T_c = 36°C) 60 min after IL-1 $beta$ producedmarked IBAT sympathoexcitation, whereas application of eitherstimulus alone did not alter the level of IBAT SND. Renal SNDresponses to the combination of IL-1 $beta$ and mild hypothermia, IL-1 $beta$ alone, and mild hypothermia alone did not differ. Second, increasesin IBAT SND were significantly higher during sustained hypothermia(T_c = 35.5°C for 120 min) and in response to an additional reductionin T_c (from 35.5 to 35°C) after sustained hypothermia in IL-1 $beta$ -treatedrats compared with saline-treated rats. In contrast, renal SNDresponses to IL-1 $beta$ and sustained hypothermia were similar in ratstreated with IL-1 $beta$ and saline. These results demonstrate thatIL-1 $beta$ alters IBAT (but not renal) SND responses to acute and sustainedhypothermia.

IL-1 $beta$ plays a key role in mediating many of the diverse physiological responses of the acute phase reaction, including fever,aphagia, activation of the hypothalamic-pituitary-adrenal axis,and activation of the sympathetic nervous system (1). Changingthe level of activity in peripheral sympathetic nerves in responseto various stimuli is an important way that physiological homeostasisis maintained. Importantly, the function of central sympatheticneurons responsible for efferent SND depends on the continuousmodulation of neuronal excitability in response to different physiologicalstates. Because immune system products influence numerous physiologicalresponses that require the integrative action of the central nervoussystem (1, 4, 27) and because the sympathetic nervoussystem can be substantially modulated by changes in the physiologicalstatus of the animal, we hypothesized that IL-1 $beta$ might play arole as a neuromodulator in sympathetic nerve regulation. Thecurrent results support this hypothesis and demonstrate targetorgan selectivity in the neuromodulatory effect of IL-1 $beta$ on efferentSND.

Because the neuromodulatory effect of IL-1 $beta$ on IBAT SND was demonstrated using direct recordings of IBAT SND, the currentresults do not address any potential interaction among IL-1 $beta$ ,hypothermia, and the sympathetic nervous system at the level ofthe tissue or neuroeffector junction. However, because peripheralSND recordings provide a window into the functional status ofcentral sympathetic neural circuits, we speculate that the observedneuromodulatory effect is mediated by interactions among IL-1 $beta$ ,hypothermia, and sympathetic premotor neurons. It must be noted,however, that modulation at the level of the sympathetic ganglioncannot be discounted because postganglionic IBAT SND recordingswere completed. Although sympathetic neural circuits are containedin spinal, brain stem, and forebrain sites (31, 33), recentstudies by Morrison (20, 21) demonstrate that the rostralraphe pallidus is involved in regulation of IBAT SND in anesthetizedrats. The role of this brain stem nucleus in mediating the neuromodulatoryrole of IL-1 $beta$ on IBAT SND remains to be determined. In addition,how this nucleus or others contained in sympathetic neural networksinteract with central sites involved in mediating the effectsof cytokines on the hypothalamic-pituitary-adrenal axis (5,6, 35) is notknown.

IL-1 $beta$ was administered in the current study because this cytokine alters the level of efferent SND (16, 28, 32), increasessplenic blood flow (26), and has been used to elucidate thecentral neural pathways subserving cytokine-induced effects onneuroendocrine neurons (5-7). The dose of IL-1 $beta$ used in the presentstudy was similar to that used in previous studies (5, 6,16, 26, 28, 32) that have documented physiological effectsof intravenous IL-1 $beta$ . On the basis of the body weight and theestimated blood volume (25) of the rats used, we estimate thatthe dose of IL-1 $beta$ in the present study produced peak plasma concentrationsof 4,000-5,000 pg/ml, similar to those produced after intraperitonealadministration of lipopolysaccharide (36), a widely acceptedmodel for systemic bacterial infection. However, circulating levelsof IL-1 $beta$ remain elevated for up to 24 h after systemic lipopolysaccharideadministration (36), whereas the half-life for elimination ofIL-1 $beta$ after intravenous injection has been reported to be <1 h(24). We suggest that the acute intravenous IL-1 $beta$ injectionparadigm is relevant in some aspects, but is not identical toan established animal model of systemic bacterial infection. Nonetheless,the current results demonstrate that, in addition to alteringthe level of sympathetic nerve activity, an additional importantmechanism by which IL-1 $beta$ influences sympathetic nerve regulationis to modulate SND responses to acutestress.

	ACKNOWLEDGEMENTS

This research was supported by National Heart, Lung, and Blood Institute Grant HL-65346.

	FOOTNOTES

Address for reprint requests and other correspondence: M. J. Kenney, Dept. of Anatomy and Physiology, Coles Hall Rm. 228,Kansas State Univ., 1600 Denison Ave., Manhattan, KS 66506 (E-mail:Kenny{at}vet.ksu.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 6 June 2001; accepted in final form 8 August 2001.

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Articles by Fels, R. J.

				N. Lu, Y. Wang, F. Blecha, R. J. Fels, H. P. Hoch, and M. J. Kenney Central interleukin-1beta antibody increases renal and splenic sympathetic nerve discharge Am J Physiol Heart Circ Physiol, May 1, 2003; 284(5): H1536 - H1541. [Abstract] [Full Text] [PDF]

				M. J. Kenney, F. Blecha, Y. Wang, R. McMurphy, and R. J. Fels Sympathoexcitation to intravenous interleukin-1beta is dependent on forebrain neural circuits Am J Physiol Heart Circ Physiol, August 1, 2002; 283(2): H501 - H505. [Abstract] [Full Text] [PDF]

				M. J. Kenney, F. Blecha, R. J. Fels, and D. A. Morgan Altered frequency responses of sympathetic nerve discharge bursts after IL-1beta and mild hypothermia J Appl Physiol, July 1, 2002; 93(1): 280 - 288. [Abstract] [Full Text] [PDF]

Interleukin-1 alters brown adipose tissue but not renal sympathetic nerve responses to hypothermia

Interleukin-1 $beta$ alters brown adipose tissue but not renal sympathetic nerve responses to hypothermia