Role of intrarenal alpha 2-adrenoceptors in the renal responses to xylazine in rats

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Role of intrarenal $alpha$ ₂-adrenoceptors in the renal responses to xylazine in rats

Rubia G. Menegaz¹, Daniel R. Kapusta², and Antonio M. Cabral¹

¹ Department of Physiological Sciences, Federal University of Espirito Santo, Vitoria, Espirito Santo, Brazil 29040-090; and ² Department of Pharmacology and Experimental Therapeutics, Louisiana State University Health Sciences Center, New Orleans, Louisiana 70112

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

This study examined the contribution of intrarenal $alpha$ ₂-adrenoceptor mechanisms to the enhanced urine flow rate (V) and urinarysodium excretion (U_NaV) responses in ketamine-xylazine-anesthetizedrats. Ten minutes after left renal artery (LRA) injection, the $alpha$ ₂-adrenoceptor antagonist yohimbine (5 µg) significantly decreasedV from 58 ± 8 to 35 ± 7 µl · min¹ · g kidney wt¹ and U_NaV from 2.8 ± 0.4 to 2.1 ± 0.4 µeq · min¹ · g kidney wt¹ without altering right kidney function. The renal effects ofthe LRA injection of yohimbine were completely abolished in chronicbilaterally renal-denervated (RDNX) rats. In RDNX rats, a higherLRA dose of yohimbine (15 µg) significantly reduced left and rightkidney V, with no effects on U_NaV. In separate bladder-catheterizedrats, yohimbine (0.5 mg/kg), 20 min after intravenous injection,significantly decreased V from 63 ± 9 to 13 ± 2 µl · min¹ · g kidney wt¹and U_NaV from 4.5 ± 0.5 to 1.1 ± 0.1 µeq · min¹ · g kidney wt¹. In RDNX rats, this dose of yohimbine reduced V and U_NaV, butthe magnitude was blunted compared with intact rats. In contrast,0.1 mg/kg iv yohimbine significantly reduced V and U_NaV to similarmagnitudes in intact and RDNX groups. Together, these findingsindicate that intravenous xylazine acts by renal nerve-dependentand -independent mechanisms to enhance renal excretory functionin ketamine-anesthetized rats. Because the effects of the LRAdose of yohimbine were abolished in renal-denervated animals,it appears that xylazine has a direct renal action to augmentthe renal excretion of water and sodium via a presynaptic $alpha$ ₂-adrenoceptorpathway that inhibits the release of neurotransmitters from renalsympathetic nerveterminals.

ketamine; yohimbine; urine flow rate; urinary sodium excretion; renal sympathetic nerves; renal excretory function; kidney

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

THE ADMINISTRATION OF $alpha$ ₂-adrenoceptor agonists (e.g., clonidine, guanabenz, etc.) produces an increase in urine flow rateand urinary sodium excretion in conscious and anesthetized animalsand humans (4, 20, 33, 36-38). The diuretic and natriureticresponses produced by $alpha$ ₂-adrenoceptor agonists result in partfrom an action of these compounds within the central nervous system(CNS) (8, 15, 16, 31). In addition, $alpha$ ₂-adrenoceptor agonistscan affect the renal handling of water and sodium via a directrenal action. In regards to this possibility, $alpha$ ₂-adrenoceptoragonists enhance the renal excretion of water by antagonizingthe hydrosmotic effects of vasopressin in the distal nephron (13,18, 32). At the cellular level, $alpha$ ₂-adrenoceptor agonists caninhibit vasopressin-stimulated cAMP formation (3, 10, 19,21, 30, 40) and thereby prevent aquaporin-mediated waterreabsorption (29, 39). In contrast to the renal handling ofwater, $alpha$ ₂-adrenoceptor agonists may act within the kidneys bya pathway independent of vasopressin to produce natriuresis (2,5, 17, 26, 27). In support of this premise, Blandfordand Smyth (5) demonstrated that the intrarenal artery infusionof low doses of clonidine selectively increased water but notelectrolyte excretion. In contrast, higher doses of clonidinewere required to increase urinary sodium and potassium excretion(5).

Similar to the renal responses produced by clonidine and guanabenz, we recently demonstrated that the $alpha$ ₂-adrenoceptor agonistxylazine produces a diuretic and natriuretic response in ketamine-anesthetizedrats (8, 9). The enhanced and sustained renal responsesattained in ketamine-anesthetized rats receiving xylazine infusionare in marked contrast to the low renal excretory levels of waterand sodium observed in rats anesthetized with ketamine or pentobarbitalsodium alone (9). In regards to the site of action, the enhancedlevel of urine flow rate, but not sodium excretion, was reducedby ~50% by the intracerebroventricular or hypothalamic paraventricularnucleus (PVN) microinjection of the $alpha$ ₂-adrenoceptor antagonistyohimbine (8). In contrast, the intravenous bolus injectionof yohimbine (but not prazosin) completely reversed both renalexcretory responses. Thus it appears that the enhanced renal excretoryresponses produced by xylazine infusion in ketamine-anesthetizedrats are mediated by complex central and peripheral $alpha$ ₂-adrenoceptoradrenergicmechanisms.

The present study was performed to investigate the contribution of intrarenal $alpha$ ₂-adrenoceptor mechanisms in mediating theenhanced renal excretory responses produced by the intravenousinfusion of xylazine in ketamine-anesthetized rats. For this purpose,studies were performed in which yohimbine was injected into theleft renal artery of ketamine- and xylazine-anesthetized rats.Changes in renal excretory function produced by yohimbine werethen compared between left (experimental) and right (control)kidneys. As demonstrated in previous studies, $alpha$ ₂-adrenoceptoragonists can affect the renal excretion of water and/or sodiumvia a pathway that involves the renal sympathetic nerves (17,26-28). Therefore, studies were also performed in chronic bilaterallyrenal-denervated rats to examine the role of an intact renal innervationin mediating the renal responses to intravenous xylazineinfusion.

	METHODS

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Experiments were performed on male Wistar rats weighing 250-300 g obtained from the Federal University of Espírito Santo.The animals were housed in a temperature- and humidity-controlledroom (25°C) with a 12-h light cycle beginning at 0700. Food (standardrat chow) and tap water were provided ad libitum. All experimentswere conducted in accordance with our institution's guide forthe care and use of experimental animals and the Brazilian PhysiologicalSociety's principles for research involvinganimals.

Surgical procedures. The anesthesia and surgery procedures used for studying the renal excretory responses produced by theintravenous infusion of xylazine in ketamine-anesthetized ratshave been previously described (8, 9). Briefly, on the dayof the experiment, rats were initially anesthetized with thiopentalsodium (Thiopental, 50 mg/kg ip supplemented intravenously asneeded, Cristalia, São Paulo, Brazil). In contrast to previousstudies (8, 9), thiopental was substituted for sodium methohexital(Brevital) due to a difficulty in obtaining the latter anesthesia.Animals were then implemented with catheters (PE-50 fused to PE-10)in the left femoral artery for the recording of arterial pressureand heart rate and the left femoral vein for the administrationof drugs and isotonic saline. As a standard procedure in our laboratory,the catheters were tunneled subcutaneously to the back of theneck. After the catheters were implanted, the rats were administeredketamine (40 mg/kg iv) over a 5-min period. An intravenous infusion(55 µl/min) of isotonic saline containing ketamine (1 mg · kg¹ · min¹) and xylazine (50 µg · kg¹ · min¹) was then started and continued throughout the experiment. Ketamine-and xylazine-anesthetized rats were then allowed at least 120min for equilibration of urine flow rate and urinary sodium excretion.For certain studies in which yohimbine was injected as an intravenousbolus, a bladder catheter (flanged PE-240) was implanted for collectionof urine. For investigations involving the intrarenal artery injectionof vehicle or antagonist, the left kidney was exposed by a leftflank incision, and the left and right ureters were isolated andcatheterized (PE-10) near the renal pelvis for collection of urine(23). A 30-gauge needle (90° bend) was advanced into the renalartery though the abdominal aorta for intrarenal administrationof yohimbine orsaline.

Certain studies were performed on rats in which the influence of the renal nerves on renal excretory function was removed.For this purpose, rats underwent chronic bilateral renal denervation5 to 7 days before the experiment (12). Briefly, under pentobarbitalsodium anesthesia, the left kidney was exposed via a flank incision.The adventitia surrounding the renal artery and vein were stripped,and all visible renal nerves were cut under a microscope (D. F.Vasconcellos 18140, São Paulo, Brazil). The vessels were thentreated with an alcohol solution containing phenol (10%). Afterrenal denervation was completed, the flank incision was suturedclosed and the procedure was repeated on the opposite side todenervate the right kidney. This renal denervation procedure preventsthe renal vasoconstrictor response to suprarenal lumbar sympatheticnerve stimulation, prevents the antinatriuretic response to environmentalstress, and reduces renal tissue norepinephrine concentrationto <5% of control for up to 15 days postdenervation (12). Ourlaboratories have previously verified that this renal denervationprocedure completely removes the influence of the renal nerveson kidney function (24, 22).

Experimental protocols. In previous studies, we have shown that in ketamine-anesthetized rats the intravenous infusion ofxylazine significantly increases urine flow rate and urinary sodiumexcretion (8, 9). The enhanced levels of these renal excretoryparameters tended to stabilize ~120 min after the start of druginfusion and remained relatively constant for an additional 90min (longer time control periods not studied) (8, 9). Therefore,in the experimental protocols described below, rats were allowedto stabilize for at least 2 h after starting the intravenous ketamineand xylazine infusion before starting the experiment. Throughoutthe experiment, mean arterial pressure and heart rate were continuouslyrecorded using a polygraph (Sensormedics Dynograf Recorder R711).

Effects of intrarenal yohimbine administration on renal excretory function in intact and bilaterally renal-denervated rats.Experiments were performed to examine the contribution of intrarenal $alpha$ ₂-adrenoceptor mechanisms to the enhanced renal excretory responseselicited by the intravenous infusion of xylazine in ketamine-anesthetizedrats (n = 8). After the stabilization of urine flow rate and urinarysodium excretion, two consecutive 10-min control urine sampleswere collected from the catheters implanted in the left and rightureters. After these control periods, yohimbine was injected intoleft renal artery (5 µg total/5 µl isotonic saline) over 3 min.Immediately after the intrarenal drug injection, five consecutiveexperimental urine samples (10 min each) were collected from theleft (experimental) and right (control)kidneys.

Studies were performed to investigate the role of intact renal nerves in mediating the renal responses produced by left renalartery injection of yohimbine (5 µg total) in ketamine- and xylazine-anesthetizedrats. For these studies, the above-mentioned protocol was repeatedin the rats (n = 7) having undergone chronic bilateral renal denervation5 to 7 days before investigation. In additional studies, changesin the left and right kidney functions produced by left renalartery administration of a higher dose of yohimbine (15 µg total/15µl isotonic saline) were examined in renal-denervated rats (n=5).

In a separate group of ketamine- and xylazine-anesthetized rats (n = 7), the same experimental protocol was repeated, withthe exception that yohimbine (5 µg) was injected as an intravenousbolus. These studies served as an additional control to verifythat the renal responses produced by left renal artery administrationof yohimbine resulted from an intrarenal action of the drug andto further demonstrate the stability of the cardiovascular andrenal excretory parameters under the time course of thestudy.

Effects of intravenous yohimbine administration on renal excretory function in intact and bilaterally renal-denervated rats.Experiments were performed to determine the effects of an intravenousbolus injection of yohimbine on the enhanced renal responses producedby an intravenous xylazine infusion in ketamine-anesthetized ratswith the intact renal innervation. After the equilibration andstabilization of the renal excretory functions, two consecutivecontrol urine samples were collected (10 min each). Yohimbine(0.5 mg/kg, n = 5; 0.1 mg/kg, n = 6), was then administered asan intravenous bolus. After waiting 10 min for the drug distribution,six consecutive experimental urine samples (10 min each) werecollected.

In additional studies, the above experimental protocol was repeated in which yohimbine (0.5 mg/kg, n = 5; 0.1 mg/kg, n = 6)was administered as an intravenous bolus to chronic bilaterallyrenal-denervatedrats.

At the end of each experiment, the kidneys were removed, decapsulated, and weighed to normalize urinary excretory data pergram of kidneyweight.

Analytic procedures and statistics. Urine volume was determined gravimetrically. Urine sodium concentration was measured byflame photometry (Micronal B262, São Paulo, Brazil). The datawere statistically analyzed using repeated-measures ANOVA andTukey's test for pairwise comparisons among the means. Statisticalsignificance was defined as P < 0.05.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Figure 1 shows the systemic cardiovascular and renal excretory effects produced by the administration of yohimbine (5 µg/5µl) into the left renal artery of ketamine- and xylazine-anesthetizedrats with intact kidneys. Consecutive urine samples (10 min each)were collected before (C1, C2) and after the yohimbine injection(over 3 min) from the left (experimental) and right (control)kidneys. The intrarenal yohimbine injection produced an immediate,but transient, decrease in the left kidney urine flow rate (C2,53 ± 8; 10 min, 35 ± 7 µl · min¹ · g kidney wt¹) and urinary sodium excretion (C2, 3.0 ± 0.4; 10 min, 2.1 ± 0.4µeq · min¹ · g kidney wt¹). In contrast, renal excretory function from the right kidneywas not altered by the injection of 5 µg of yohimbine into theleft renal artery. In preliminary studies, left renal artery injectionof isotonic saline vehicle (5 or 15 µl over 3 min) did not alterany cardiovascular or renal excretory (left or right kidney) parameter(data not shown).

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Fig. 1. Effects of left renal artery yohimbine injection on cardiovascular and renal excretory function in ketamine- and xylazine-anesthetized Wistar rats with intact renal innervation. Values are means ± SE illustrating cardiovascular and renal responses produced by left renal artery injection of $alpha$ ₂-adrenoceptor antagonist yohimbine (5 µg total) in 8 rats anesthetized with ketamine (40 mg/kg iv bolus over 5 min) and infused (55 µl/min) with isotonic saline containing ketamine (1 mg · kg¹ · min¹) and xylazine (50 µg · kg¹ · min¹). Urine samples were collected from left (

, experimental) and right ( $open circle$ , control) kidneys during control (C1-C2, 10 min each) and immediately after left renal artery yohimbine injection (over 3 min) (consecutive 10-min urine samples for 50 min). HR, heart rate; MAP, mean arterial pressure; V, urine flow rate; U_NaV, urinary sodium excretion; bpm, beats per minute; gKw, grams kidney weight. * P < 0.05, significantly different from corresponding control.

In contrast to the findings shown in Fig. 1, renal excretory function from both kidneys remained unchanged after left renalartery injection of yohimbine (5 µg total) in ketamine- and xylazine-anesthetizedrats that underwent chronic bilateral renal denervation (Fig.2). Mean arterial pressure and heart rate were not altered byleft renal artery injection of yohimbine in intact (Fig. 1) orbilaterally renal-denervated rats (Fig. 2). Moreover, in additionalstudies (data not shown), the intravenous bolus administrationof the same dose of yohimbine (5 µg total) did not affect systemiccardiovascular or renal excretory function in ketamine- and xylazine-anesthetizedrats with an intact renal innervation. These latter findings andthe results depicted in Fig. 2 demonstrate the stability of thecardiovascular and renal excretory parameters over the time courseof the study. Moreover, these findings indicate that the renalresponses produced by left renal artery injection of yohimbine(Fig. 1) occur via an intrarenal action that is dependent on anintact renal innervation.

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Fig. 2. Effects of left renal artery yohimbine injection on cardiovascular and renal excretory function in ketamine- and xylazine-anesthetized Wistar rats with bilateral renal denervation (DNX). Values are means ± SE illustrating cardiovascular and renal responses produced by left renal artery injection of 5 µg total of yohimbine in 7 chronic bilaterally renal-denervated rats anesthetized with ketamine and xylazine. Experiments were performed during continuous intravenous infusion of isotonic saline (55 µl/min) containing ketamine (1 mg · kg¹ · min¹) and xylazine (50 µg · kg¹ · min¹). Consecutive 10-min urine samples were collected from the left (

, experimental) and right kidney ( $open circle$ , control) during control (C1-C2) and immediately after left renal artery injection of yohimbine (5 µg total over 3 min) (time points 10-50 min).

Figure 3 shows the cardiovascular and renal responses produced by left renal artery injection of a higher dose of yohimbine(15 µg total) in ketamine- and xylazine-anesthetized rats withbilaterally renal-denervated kidneys. Compared with respectivecontrol levels for each kidney, left renal artery injection of15 µg yohimbine did not alter urinary sodium secretion in eitherkidney (Fig. 3). These findings are similar to those shown inFig. 2, demonstrating that the antinatriuretic response to 5 µgyohimbine (Fig. 1) is abolished in renal-denervated rats (Fig.2). In contrast to the effects on urinary sodium excretion, leftrenal artery injection of 15 µg yohimbine decreased urine flowrate from left and right kidneys of renal-denervated rats (Fig.3). Note that a significant decrease in urine flow rate was notobserved when a lower dose (5 µg) of yohimbine was injected intothe left kidney of renal-denervated rats (Fig. 2). Mean arterialpressure and heart rate were not altered by this higher intrarenaldose of yohimbine.

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Fig. 3. Effects of high dose left renal artery yohimbine injection on cardiovascular and renal excretory function in ketamine- and xylazine-anesthetized Wistar rats with bilateral renal denervation. Values are means ± SE illustrating cardiovascular and renal responses produced by left renal artery injection of yohimbine (15 µg total) in 5 chronic bilaterally renal-denervated rats anesthetized with ketamine and xylazine. Experiments were performed during continuous intravenous infusion of isotonic saline (55 µl/min) containing ketamine (1 mg · kg¹ · min¹) and xylazine (50 µg · kg¹ · min¹). Consecutive 10-min urine samples were collected from left (

, experimental) and right kidney ( $open circle$ , control) during control (C1-C2) and immediately after left renal artery injection of yohimbine (15 µg total over 3 min) (time points 10-50 min). $tau$ ,* P < 0.05, significantly different from corresponding control.

Figure 4 illustrates the cardiovascular and renal responses produced by the intravenous bolus injection of yohimbine (0.5mg/kg) in intact (n = 5) and chronic bilaterally renal-denervatedrats (n = 5). For these studies, consecutive urine samples (10min) were collected from ketamine- and xylazine-anesthetized ratsimplanted with a urinary bladder catheter. Compared with respectivecontrol values (C1, C2), the intravenous administration of yohimbine(0.5 mg/kg) produced an immediate and profound decrease in urineflow rate and urinary sodium excretion in rats with intact anddenervated kidneys. Despite these similar effects, the magnitudeof the decrease in urine flow rate and urinary sodium excretionproduced by yohimbine was significantly blunted (P < 0.05) inrenal-denervated rats compared with intact rats. Intravenous yohimbineproduced a statistically significant difference in the heart rate(tachycardia) but not in the blood pressure response between intactand renal-denervated groups.

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Fig. 4. Cardiovascular and renal excretory responses produced by intravenous bolus administration of yohimbine in ketamine- and xylazine-anesthetized Wistar rats. Values are means ± SE illustrating cardiovascular and renal responses produced by intravenous bolus injection of yohimbine (0.5 mg/kg) in intact (

, n = 5) and bilaterally renal-denervated ( $open circle$ , n = 5) rats anesthetized with ketamine and xylazine. Experiments were performed during continuous intravenous infusion of isotonic saline (55 µl/min) containing ketamine (1 mg · kg¹ · min¹) and xylazine (50 µg · kg¹ · min¹). Consecutive 10-min urine samples were collected from a urinary bladder catheter during control (C1-C2) and 10 min after intravenous injection of yohimbine (0.5 mg/kg) (time points 20-70 min). * P < 0.05, significantly different from intact group at corresponding time point.

Figure 5 shows the systemic cardiovascular and renal excretory effects produced by the intravenous bolus administration of0.1 mg/kg yohimbine in ketamine- and xylazine-anesthetized rats.It should be emphasized that this is a dose five times lower thanthat used in studies depicted in Fig. 4. Compared with respectivepredrug control levels (C1, C2), 0.1 mg/kg iv yohimbine produceda marked decrease in urine flow rate and urinary sodium excretionin rats with intact and denervated kidneys (Fig. 5). Note, however,that the magnitude decrease in each renal excretory parameterwas similar between intact and renal-denervated groups (Fig. 5).This finding differs from those shown in Fig. 4 in that the intravenousinjection of 0.5 mg/kg yohimbine reduced urine flow rate and urinarysodium excretion to a greater degree in intact than in renal-denervatedanimals. In fact, the renal responses produced by 0.5 mg/kg yohimbinein renal-denervated rats (Fig. 4) were of similar magnitude tothose produced by the injection of 0.1 mg/kg in either intactor denervated rats (Fig. 5). Finally, the intravenous bolus administrationof 0.1 mg/kg yohimbine did not produce a statistically significantchange in the heart rate or mean arterial pressure response betweengroups.

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Fig. 5. Cardiovascular and renal excretory responses produced by intravenous bolus administration of low dose yohimbine in ketamine- and xylazine-anesthetized Wistar rats. Values are means ± SE illustrating cardiovascular and renal responses produced by intravenous bolus injection of yohimbine (0.1 mg/kg) in intact (

, n = 6) and chronic bilaterally renal-denervated ( $open circle$ , n = 6) rats anesthetized with ketamine and xylazine. Experiments were performed during continuous intravenous infusion of isotonic saline (55 µl/min) containing ketamine (1 mg · kg¹ · min¹) and xylazine (50 µg · kg¹ · min¹). Consecutive 10-min urine samples were collected from a urinary bladder catheter during control (C1-C2) and 10 min after intravenous injection of yohimbine (0.1 mg/kg) (time points 20-70 min).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The findings of the present study demonstrate that $alpha$ ₂-adrenoceptor mechanisms within the kidneys are activated and contributeto the diuretic and natriuretic responses produced by the intravenousinfusion of xylazine in ketamine-anesthetized rats. As shown inprevious studies, a component of the enhanced diuretic responsealso occurs as a result of xylazine's action to inhibit the secretion-releaseof arginine vasopressin by stimulating $alpha$ ₂-adrenoceptors in theCNS, particularly in the hypothalamic PVN (8). Together, thesefindings indicate that the enhanced and sustained increase inurine flow rate and urinary sodium excretion produced by the intravenousxylazine infusion are mediated via activation of complex centraland peripheral $alpha$ ₂-adrenoceptorpathways.

In previous studies, we showed that the intravenous bolus injection of yohimbine (0.5 mg/kg) produces a near complete reversalof the enhanced renal excretory responses produced by intravenousxylazine infusion in ketamine-anesthetized rats (9). In contrast,the intravenous bolus administration of prazosin (0.5 mg/kg),a selective $alpha$ ₁-adrenoceptor antagonist, was without effect. Althoughthese observations clearly demonstrate the involvement of $alpha$ ₂-adrenoceptorpathways in mediating the enhanced renal responses, they do notprovide information as to the site(s) of action ofxylazine.

In the present studies, left renal artery injection of 5 µg total of yohimbine significantly reduced urine flow rate and urinarysodium excretion in the experimental (left) but not in the control(right) kidney of ketamine- and xylazine-anesthetized rats. Comparedwith predrug control levels, the renal excretion of water andsodium from the left kidney was reduced by 34 and 30%, respectively.In contrast, the intravenous bolus injection of yohimbine at thesame dose (5 µg total) did not alter renal excretory functionin either kidney. Together, these results suggest that intrarenal $alpha$ ₂-adrenoceptor mechanisms are activated and contribute to theenhanced diuretic and natriuretic responses produced by xylazineinfusion.

In related studies, Blandford and Smyth (5) demonstrated that the intrarenal infusion of clonidine produced a dose-relatedincrease in urine flow rate. In their studies, however, an increasein urinary sodium excretion and an increase in osmolar clearancewere only observed at the highest infusion rate tested (5).Thus these investigators concluded that different mechanisms mightbe involved in mediating the dissociated effects of clonidineon water and sodium excretion. The concept that two independentmechanisms may mediate the effects of $alpha$ ₂-adrenoceptor agonistson the renal excretion of sodium and water has previously beensuggested (36, 37). In regards to mechanisms, Blandford andSmyth (5) proposed that clonidine may have acted within thekidneys to stimulate inhibitory presynaptic $alpha$ ₂-adrenoceptors andthereby reduce norepinephrine release from renal sympathetic nerveterminals. The inhibition of norepinephrine release would promotewater and sodium excretion by reducing the activity of postjunctional $alpha$ ₁- adrenoceptors located on the renal tubules and vasculature(11, 16, 34). In agreement with this concept, the resultsof the present studies indicate that the intrarenal administrationof yohimbine blunted the enhanced renal responses to intravenousxylazine by a pathway that involves the renal nerves. This wasdemonstrated by the observation that the renal artery injectionof 5 µg total of yohimbine failed to alter the enhanced diureticand natriuretic responses produced by intravenous xylazine inbilaterally renal-denervated rats (Fig. 2). From these findings,it may be proposed that in intact rats an intrarenal componentof the diuresis and natriuresis produced by intravenous xylazineinfusion is mediated by the stimulation of presynaptic $alpha$ ₂-adrenoceptorslocated on renal nerve terminals. Activation of presynaptic $alpha$ ₂-adrenoceptorson renal sympathetic nerve terminals would inhibit the neuralrelease of norepinephrine and promote water and sodium excretion,responses that are reversed by the renal artery administrationofyohimbine.

In addition to a pathway involving the renal nerves, xylazine may increase urine flow rate in ketamine-anesthetized rats byactivating $alpha$ ₂-adrenoceptors in the collecting ducts. Along theselines, other $alpha$ ₂-adrenoceptor agonists (e.g., clonidine, rilmelnidine,etc.) have been shown to enhance urine output by inhibiting therenal tubular effects of vasopressin on water transport (6,7, 14, 18, 35). To test this possibility under our experimentalconditions, we examined whether a higher intrarenal artery doseof yohimbine could reverse the enhanced levels of urine flow ratethat are observed in renal-denervated ketamine- and xylazine-anesthetizedrats. Chronic bilaterally renal-denervated rats were used in theseinvestigations to specifically study the role of renal tubular $alpha$ ₂-adrenoceptor pathways in mediating the effects of yohimbine(and thus xylazine) on renal excretoryfunction.

In these studies, left renal artery injection of 15 µg of yohimbine significantly reduced urine flow rate from both the leftand right denervated kidneys (Fig. 3). Of interest, this higherintrarenal dose of yohimbine did not alter urinary sodium excretionin either the left or right denervated kidney. On the basis ofthese observations, it is clear that intact renal nerves are ofparticular importance in mediating the effects of yohimbine andxylazine on the renal handling of sodium. In contrast, becauseintrarenal yohimbine markedly reduced the enhanced level of urineflow rate in renal-denervated rats, it appears that xylazine mayenhance urine flow rate via activating postjunctional $alpha$ ₂-adrenoceptorsin the distal tubules. Although these observations suggest thispossibility, it should be emphasized that the present findingsdo not specifically prove this point. This stems from the findingthat left renal artery injection of 15 µg of yohimbine reducedurine flow rate in both kidneys, thereby indicating that the responsesobserved in the right kidney occurred subsequent to a leakageinto the peripheral circulation. Thus yohimbine may have causeda decrease in urine flow rate in both kidneys via an extrarenalmechanism.

On the basis of the present findings from the intrarenal artery yohimbine studies, it would be predicted that the renal nerves(and thus the intrarenal neuronal release of norepinephrine) arealso involved in mediating a component of the renal responsesproduced by the systemic intravenous administration of yohimbine.In fact, this was shown to be the case because the reduction inurine flow rate and urinary sodium excretion produced by the intravenousbolus injection of yohimbine (0.5 mg/kg) in renal-denervated ratswas less pronounced than that observed in intact rats (Fig. 4).Of further interest was the observation that when yohimbine wasadministered as an intravenous bolus at a dose five times lower(0.1 mg/kg), the reduction magnitude in both renal excretory parameterswas blunted and remarkably similar between the groups of ratswith intact and denervated kidneys (Fig. 5). In these studies,the injection of 0.1 mg/kg of yohimbine to intact and renal-denervatedrats (Fig. 5) produced a pattern of renal responses that werecomparable to those evoked by a high dose of yohimbine (0.5 mg/kg)in bilaterally renal-denervated rats (Fig. 4).

Perspectives

The ketamine-xylazine protocol provides a novel approach to study the $alpha$ ₂-adrenergic control of renal function (8, 9).In addition to a direct renal action (present findings), it isapparent that other nonrenal mechanisms also contribute in mediatingthe renal responses to this $alpha$ ₂-adrenoceptor agonist. For instance,the pattern (magnitude and time course) of the renal responsesproduced by the intravenous bolus injection of 0.5 and 0.1 mg/kgyohimbine may be due to variance in the ability of these dosesto effectively antagonize xylazine at central $alpha$ ₂-adrenoceptors.This is important because stimulation of $alpha$ ₂-adrenoceptors in theCNS is known to produce renal sympathoinhibition and thereby reducerenin release, renal tubular reabsorption of sodium and water,and renal vascular resistance (1, 8, 11). In the CNS microinjectionstudies, we previously demonstrated that during intravenous infusion,xylazine activates central mechanisms to enhance the renal excretionof sodium and water (8). In intact rats, the high dose (0.5mg/kg iv) of yohimbine may have crossed the blood-brain barrierin a sufficient concentration to gain access to brain regions(e.g., rostroventrolateral medulla; 23, 25, 31) where it effectivelyantagonized the central sympatholytic effects of xylazine. Onrestoration of sympathetic outflow to the kidneys, an increasein renal tubular sodium retention would occur, thereby producinga marked reduction in urine flow rate and urinary sodium excretion.In contrast to this action, it is likely that the low dose ofyohimbine (0.1 mg/kg iv) did not gain access into the CNS in asufficient concentration to effectively prevent the sympatholyticaction of xylazine. Thus the renal responses to the low dose ofyohimbine may be mediated by other extrarenal mechanisms (e.g.,adrenal gland, etc.). As a consequence, the renal sympathoinhibitoryeffect of xylazine would still predominate and prevent the fullreversal of the enhanced renal responses produced by the intravenousyohimbine injection. The profound hypotensive (but only modesttachycardia) response produced by the intravenous bolus injectionof 0.1 mg/kg of yohimbine in intact rats (Fig. 5) also providessupport to indicate a blockade of peripheral (vascular) but notcentral $alpha$ ₂-adrenoceptors. Finally, the observation that renalexcretory function was augmented in chronic bilaterally renal-denervatedrats (partially reversed by yohimbine) clearly reveals an $alpha$ ₂-adrenoceptoraction of xylazine that is independent of the renal nerves. Furtherstudies using the ketamine-xylazine model may help to elucidatethe sites and mechanisms by which these interesting renal nerve-independentresponses aremediated.

In summary, the present investigations indicate that intrarenal $alpha$ ₂-adrenoceptor mechanisms are involved in mediating a componentof the enhanced renal excretory responses produced by the intravenousinfusion of xylazine in ketamine-anesthetized rats. The intrarenaleffects of xylazine on the renal handling of sodium and waterare mediated in part by a pathway that involves the renal sympatheticnerves. This could occur via the action of xylazine to activatepresynaptic inhibitory $alpha$ ₂-adrenoceptors to inhibit the renal nerveterminal release ofnorepinephrine.

	ACKNOWLEDGEMENTS

This work was supported by grants from the Council for Science and Technology to A. M. Cabral and R. G. Menegaz and from theNational Institute of Diabetes and Digestive and Kidney Diseases(DK-43337 and DK-02605) to D. R.Kapusta.

	FOOTNOTES

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.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: A. M. Cabral, Universidade Federal do Espírito Santo, Departamento de Ciências Fisiológicas, Vitoria, Espirito Santo, Brazil 29040-090 (E-mail: acabral{at}npd.ufes.br).

Received 2 September 1999; accepted in final form 10 November 1999.

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