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CARDIAC, RENAL, AND RESPIRATORY INTEGRATION

Increased H₂O₂ counteracts the vasodilator and natriuretic effects of superoxide dismutation by tempol in renal medulla

Department of Physiology, Medical College of Wisconsin, Milwaukee, Wisconsin 53226

Submitted 15 October 2002 ; accepted in final form 4 June 2003

	ABSTRACT

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION DISCLOSURES REFERENCES

 
A membrane-permeable SOD mimetic, 4-hydroxytetramethyl-piperidine-1-oxyl (tempol), has been used as an antioxidant to prevent hypertension. We recently found that this SOD mimetic could not prevent development of hypertension induced by inhibition of renal medullary SOD with diethyldithiocarbamic acid. The present study tested a hypothesis that increased H₂O₂ counteracts the effects of tempol on renal medullary blood flow (MBF) and Na⁺ excretion (U_NaV), thereby restraining the antihypertensive effect of this SOD mimetic. By in vivo microdialysis and Amplex red H₂O₂ microassay, it was found that interstitial H₂O₂ levels in the renal cortex and medulla in anesthetized rats averaged 55.91 ± 3.66 and 102.18 ± 5.16 nM, respectively. Renal medullary interstitial infusion of tempol (30 µmol·min^-1·kg^-1) significantly increased medullary H₂O₂ levels by 46%, and coinfusion of catalase (10 mg·min^-1·kg^-1) completely abolished this increase. Functionally, removal of H₂O₂ by catalase enhanced the tempol-induced increase in MBF, urine flow, and U_NaV by 28, 41, and 30%, respectively. Direct delivery of H₂O₂ by renal medullary interstitial infusion (7.5-30 nmol·min^-1· kg^-1) significantly decreased renal MBF, urine flow, and U_NaV, and catalase reversed the effects of H₂O₂. We conclude that tempol produces a renal medullary vasodilator effect and results in diuresis and natriuresis. However, this SOD mimetic increases the formation of H₂O₂, which constricts medullary vessels and, thereby, counteracts its vasodilator actions. This counteracting effect of H₂O₂ may limit the use of tempol as an antihypertensive agent under exaggerated oxidative stress in the kidney.

free radicals; renal hemodynamics; renal medulla; kidney; rat

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Then this cation form of tempol directly reacts with O₂^-· to produce O₂ and regenerate tempol. In this reaction, tempol produces H₂O₂ with a rate constant of 10⁷ M-1 · s^-1 (20). As a catalyst, however, tempol concentrations remain constant; therefore, it will more efficiently remove O₂^-· than will the stoichiometric scavengers (23).

Recent studies have indicated that excessive production of reactive oxygen species contributes to the development of hypertension in different animal models (9, 27, 28). Administration of antioxidant enzymes such as SOD and catalase has been shown to prevent or treat hypertension (1, 8). However, the potential benefits of systemic administration of SOD are limited, because SOD does not permeate biological membranes and is therefore unable to remove O₂^-· produced intracellularly (5). To overcome these limitations, tempol, a membrane-permeable and metal-independent SOD mimetic, has been utilized as an antioxidant for the removal of intracellular and extracellular O₂^-·. Indeed, it has been found that arterial blood pressure could be lowered by tempol in several models of hypertension (2, 25, 27).

More recently, we reported that increased oxidative stress in the renal medulla results in a reduction of medullary blood flow (MBF) and Na⁺ retention, leading to hypertension (14). Given the vasodilator and natriuretic effect of tempol infused into the renal medulla and its chronic antihypertensive action in other models, we used this SOD mimetic to block the hypertension induced by enhanced renal medullary oxidative stress. However, chronic renal medullary infusion of tempol at a dose similar to that used in other animal models (50 µmol · kg^-1 · day^-1) failed to prevent hypertension induced by enhanced medullary oxidative stress, unless catalase was administered (14). It appears that increased H₂O₂ production by tempol in the renal medulla is counteracting vasodilator, natriuretic, and, ultimately, antihypertensive effects of tempol. The present study was designed to test this hypothesis. First, using Amplex red fluorescent spectrometry and microdialysis techniques, we determined tempol-induced H₂O₂ production in the renal medulla and the effects of the tempol-induced increase in H₂O₂ on renal MBF and Na⁺ excretion. By infusion of H₂O₂ in the renal medulla, we also examined the direct effects of H₂O₂ on the renal MBF and urinary excretion functions.

	MATERIALS AND METHODS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION DISCLOSURES REFERENCES

 
Fluorescence spectrometric assay of H₂O₂ concentrations. Fluorescence spectrometry of renal interstitial H₂O₂ levels was performed by using Amplex red (Molecular Probes, Eugene, OR). Amplex red is a fluorogenic substrate with very low background fluorescence; it reacts with H₂O₂ with a 1:1 stoichiometry to produce highly fluorescent resorufin (17). Briefly, 200 µM Amplex red reagent and 1 U/ml horseradish peroxidase were added to the renal dialysate collected from the study (50 µl) or an H₂O₂ standard solution in 50 mM sodium phosphate buffer (pH 7.4), and the sample was incubated for 30 min in Falcon 96-well microplates in the dark at room temperature. Fluorescence intensity was measured in an automatic microplate reader (model KC4, Bio-Tek Instruments, Winooski, VT) at an excitation wavelength of 530 ± 25 nm and an emission wavelength of 590 ± 35 nm. After subtraction of background fluorescence, H₂O₂ concentrations of renal interstitial dialysate were calculated on the basis of an H₂O₂ standard curve generated using H₂O₂ and Amplex red.

Animal preparation for microdialysis and renal medullary flowmetry. Male Sprague-Dawley rats (250-300 g) were purchased from Harlan Sprague Dawley (Madison, WI) and housed in the Animal Resource Center at the Medical College of Wisconsin. The rats were fed pellet diets with normal salt (1% NaCl), and water was provided ad libitum. To prepare for microdialysis, the rats were anesthetized with ketamine (Ketaject; 30 mg/kg body wt im) and thiobutabarbital (Inactin; 50 mg/kg body wt ip) and then placed on a thermostatically controlled warming table to maintain body temperature at 37°C. One catheter was placed in the left femoral vein for a continuous infusion of 0.9% NaCl solution containing 2% albumin at a rate of 3.0 ml/h throughout the experiment to replace fluid loss and maintain a constant hematocrit (40%), which was measured during equilibration or when blood samples were taken during the experiment. The left femoral artery was cannulated and connected to a Statham pressure transducer for monitoring of mean arterial pressure (MAP) throughout the experiment. The left kidney was exposed by a midline abdominal incision and placed in a stainless steel cup for implantation of microdialysis probes to dialyze H₂O₂ from the renal interstitium or for implantation of optical fibers to measure cortical and medullary blood flows (CBF and MBF, respectively), as we described previously (3, 33). After implantations, a 0.9% NaCl solution was infused continuously at a rate of 0.6 ml/h to maintain the patency of interstitial infusion until the infusions of tempol, catalase, and H₂O₂ (see protocols 1-4). Urine from the left and right kidney was collected via a ureteral catheter. The rats were allowed to stabilize after the surgical procedure for 1.5-2 h. Animals were euthanized at the end of experiments with an excess intravenous dose of pentobarbital sodium (150 mg/kg). The left kidney was excised and weighed, and the position of the dialysis probes or laser optic fibers was confirmed. If the probes or fibers were positioned incorrectly, the data of these dialysates or data for blood flow signals were discarded.

Protocol 1: effects of renal medullary interstitial infusion of tempol and catalase on renal interstitial concentrations of H₂O₂. In vivo microdialysis was performed as we described previously (3, 31). Briefly, the left kidney of anesthetized rats was immobilized by placement of its dorsal side up in a kidney cup. A microdialysis probe (Bioanalytical Systems, West Lafayette, IN) with a 0.5-mm tip diameter, 2-mm dialysis length, and 20-kDa transmembrane diffusion cutoff was gently implanted into the renal cortex (1.5 mm deep) horizontally from the kidney pole, and another was implanted into the renal medulla (5-5.5 mm deep) vertically from the dorsal surface. The cortical probe was connected to a microinfusion pump and perfused with PBS containing (in mM) 80 NaCl, 40.5 Na₂HPO₄, and 9.5 NaH₂PO₄ (pH 7.4, 300 mosM). The medullary probe was perfused with PBS containing (in mM) 205 NaCl, 40.5 Na₂HPO₄, and 9.5 NaH₂PO₄ (pH 7.4, 550 mosM) at a rate of 2.0 µl/min throughout the experiment. The microdialysis probe was also constructed with an incorporated infusion line, which could be used for renal medullary interstitial infusion during collection of the dialysate when it was implanted into the renal medulla. After a 1.5-h equilibration period, two 30-min control dialysates from the renal cortex and medulla were collected for the analysis of basal renal interstitial H₂O₂ levels. Then tempol (30 µmol · min^-1 · kg^-1) or tempol + catalase (10 mg · min^-1 · kg^-1) was infused into the renal medullary interstitium for 60 min, and two additional 30-min samples of cortical and medullary dialysates were collected. Doses of tempol and catalase for renal medullary interstitial infusions were chosen on the basis of previous in vivo studies (14, 32) showing that they can effectively reduce oxidative stress. Especially, the dose of tempol was chosen to simulate its effect on H₂O₂ production shown in our chronic experiments (14), so that a similar increase in H₂O₂ levels in the renal medulla could be reached. All dialysate samples (50 µl) were reacted with fluorescence dye (Amplex red reagent) immediately at the end of each experiment, and then the fluorescence intensity was measured in Falcon 96-well microplates as described above.

Protocol 2: effects of renal medullary interstitial infusion of tempol and catalase on MBF and renal function. The rats were anesthetized and surgically prepared as described for protocol 1. An extruded polyethylene interstitial catheter (100-µm tip diameter) was implanted into the renal medulla (5 mm deep) for interstitial infusion, and laser optical fibers (0.5-mm diameter) were implanted into the renal medulla (5-5.5 mm deep) and renal cortex (1.5 mm deep), respectively. These laser fibers were connected to laser-Doppler flowmeter probes to record blood flow signals (red cell capability x velocity), as we described previously (32, 33). After control recordings, tempol (30 µmol · min^-1 · kg^-1) was infused into the renal medullary interstitium for 60 min, and MAP and cortical and medullary laser-Doppler flow (LDF) signals were recorded throughout the experiment. In additional groups of rats, catalase (10 mg · min^-1 · kg^-1) was infused into the renal medulla 30 min before tempol infusion and continued during tempol infusion to test whether the effects of tempol could be blocked by catalase. In experiments to determine whether endogenous medullary H₂O₂ contributes to the control of water and Na⁺ excretion, urine was collected from ureteral catheters during tempol and catalase infusions. The urine samples over two 20-min periods from left and right kidneys were used to determine Na⁺ and K⁺ concentrations with a flame photometer. Urine flow rates were determined gravimetrically and used to determine electrolyte excretion rates. Urinary excretion data and renal blood flow were factored per gram kidney weight.

Protocol 3: effects of renal medullary interstitial infusion of H₂O₂ and catalase on renal interstitial concentrations of H₂O₂. To study the effects of exogenous H₂O₂ on renal blood flow and renal function, we first tested the efficiency of renal medullary infusion of H₂O₂ to increase its concentration. In vivo microdialysis was performed as described in protocol 1. After two 30-min control dialysates from the renal cortex and medulla were collected, increasing concentrations of H₂O₂ (7.5, 15, and 30 nmol · min^-1 · kg^-1) or H₂O₂ (30 nmol · min^-1 · kg^-1) + catalase (10 mg · min^-1 · kg^-1) were infused into the renal medullary interstitium for 60 min. The cortical and medullary dialysates were collected repeatedly after H₂O₂ or catalase treatment. The H₂O₂ concentrations in the dialysates were quantitated by Amplex red reagent as described above.

Protocol 4: effects of renal medullary interstitial infusion of H₂O₂ and catalase on MBF and renal function. The rats were surgically prepared, and optical fibers and ureters were implanted as described in protocol 2. MAP, CBF, and MBF were recorded throughout the experiment. After control recording, increasing doses of H₂O₂ (7.5, 15, and 30 nmol · min^-1 · kg^-1) were infused into the renal medullary interstitium for 60 min. Then catalase (10 mg · min^-1 · kg^-1) was added to the infusion solution and infused for another 60 min. During all infusion periods, MAP, CBF, and MBF were continuously recorded, and urine samples from the left and right kidneys were collected for measurement of water and Na⁺ excretion.

Statistics. Values are means ± SE. The significance of differences within and between groups in multiple groups of experiments was evaluated using an analysis of variance for repeated measures followed by Duncan's multiple range tests. P < 0.05 was considered statistically significant.

	RESULTS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION DISCLOSURES REFERENCES

 
Standard curve of the resorufin-H₂O₂ assay and H₂O₂ dialysis efficiency. As shown in Fig. 1, the fluorescence intensity produced by the reaction of Amplex red with H₂O₂ was linear for a wide range of the H₂O₂ concentrations. The minimal detectable H₂O₂ concentration was 10 nM, and the linearity of the H₂O₂ standard extended to >1 µM H₂O₂. The efficiency of H₂O₂ dialysis through BAS microdialysis probes was determined from in vitro dialysis experiments in which concentrations of H₂O₂ in the dialysates were compared with H₂O₂ concentration in the standard solution. It was found that a 96% recovery could be achieved in the effluent dialysate solution.

View larger version (17K): [in this window] [in a new window]   Fig. 1. Standard curve and regression equation of resorufin-H2O2 assay. Inset: relation of a low range of H2O2 concentrations and Amplex red fluorescence. Data were obtained from 6 independent measurements.

Effects of renal medullary interstitial infusion of tempol and catalase on renal interstitial concentrations of H₂O₂. Interstitial H₂O₂ concentrations achieved in renal cortical and medullary dialysate under control conditions and after different treatments are presented in Fig. 2. Basal H₂O₂ concentrations in the renal medulla averaged 102.18 ± 5.16 nM, which were significantly higher than 55.91 ± 3.66 nM in cortical dialysate. After interstitial infusion of tempol (30 µmol · min^-1 · kg^-1) for 60 min, H₂O₂ concentrations in renal medullary dialysates were significantly increased to 164.16 ± 11.22 nM, and H₂O₂ concentration in cortical dialysates rose to 93.04 ± 10.34 nM. In rats receiving an interstitial infusion of tempol + catalase (10 mg · min^-1 · kg^-1) for 60 min, H₂O₂ concentrations in renal cortical and medullary dialysates were reduced to levels averaging 50.58 ± 6.28 and 52.53 ± 7.86 nM, respectively. In these experiments, the increase in H₂O₂ levels in the renal medulla by acute infusion of 30 µmol · min^-1 · kg^-1 tempol was less than that found during chronic renal medullary infusion of tempol in our previous study (14).

View larger version (12K): [in this window] [in a new window]   Fig. 2. Effects of renal medullary interstitial infusion of tempol and catalase on renal interstitial concentrations of H2O2. Values are means ± SE (n = 7).*P < 0.05 vs. control; #P < 0.05 vs. cortex.

Effects of renal medullary interstitial infusion of tempol and catalase on MBF and renal function. The effects of renal medullary interstitial infusion of tempol and catalase on CBF and MBF are summarized in Fig. 3. In control periods, the LDF signals from the fibers implanted in the renal cortex and outer medulla averaged 1.12 ± 0.04 and 0.48 ± 0.01 V, respectively. Renal medullary interstitial infusion of tempol increased medullary LDF signals by a maximum of 42% compared with control values. In the presence of catalase, renal interstitial infusion of tempol had no effect on LDF signals in the cortical regions but significantly increased medullary flow signals by a maximum of 67%. Renal medullary infusion of catalase alone increased medullary LDF signals by 10% but had no effect on cortical LDF signals.

View larger version (15K): [in this window] [in a new window]   Fig. 3. Effects of renal medullary interstitial infusion of tempol on mean arterial pressure (MAP) and renal cortical and medullary blood flow in the absence or presence of catalase. LDF, laser-Doppler flow; C, control. Values are means ± SE (n = 7). *P < 0.05 vs. control; #P < 0.05 vs. tempol.

The effects of renal medullary interstitial infusion of tempol and catalase on renal function are summarized in Fig. 4. Medullary infusion of tempol increased urine flow rate and Na⁺ excretion in infused kidney by 35 and 47%, respectively. In the presence of catalase, tempol increased urine flow rate and Na⁺ excretion by a maximum of 76 and 77%, respectively. Catalase alone also increased urine flow rate and Na⁺ excretion by 12 and 16%, respectively. In the contralateral kidneys, urine flow rate and Na⁺ excretion were not significantly altered during these treatments. MAP remained unchanged throughout all the above studies.

View larger version (20K): [in this window] [in a new window]   Fig. 4. Effects of renal medullary interstitial infusion of tempol on renal function [urine flow (UV) and Na+ excretion (UNaV)] in the absence or presence of catalase. Contralateral, contralateral kidney; infused, infused kidney; kwt, kidney weight. Values are means ± SE (n = 7). *P < 0.05 vs. control; #P < 0.05 vs. tempol.

Effects of renal medullary interstitial infusion of H₂O₂ and catalase on local tissue concentrations of H₂O₂. H₂O₂ concentrations in renal cortical and medullary dialysates under control conditions and after treatments are presented in Fig. 5. After medullary interstitial infusion of H₂O₂ at 30 nmol · min^-1 · kg^-1, the highest dose used in this study for 60 min, H₂O₂ concentration in renal medullary dialysates was significantly increased from 116.23 ± 4.02 to 210.94 ± 13.2 nM, which was similar to that found during acute (see above) and chronic tempol infusion (14). In the presence of catalase, renal medullary interstitial infusion of H₂O₂ (30 nmol · min^-1 · kg^-1) did not increase H₂O₂ concentration in the renal medulla, which remained at a low level (43.46 ± 7.39 nM). H₂O₂ concentration in the cortical dialysates was not changed during renal medullary infusion of H₂O₂ alone or H₂O₂ + catalase.

View larger version (13K): [in this window] [in a new window]   Fig. 5. Effects of renal medullary interstitial infusion of H2O2 and catalase on renal interstitial concentrations of H2O2. Values are means ± SE (n = 7). *P < 0.05 vs. control; #P < 0.05 vs. cortex.

Effects of renal medullary interstitial infusion of H₂O₂ and catalase on MBF and renal function. Having determined the effects of exogenous infusions of H₂O₂ on medullary interstitial concentrations, the effects of these elevations on renal blood flow and renal functions were examined. The results of these experiments are summarized in Fig. 6. Renal medullary interstitial infusion of H₂O₂ (30 nmol · min^-1 · kg^-1) decreased medullary LDF signals by 31%. Coinfusion of H₂O₂ with catalase (10 mg · min^-1 · kg^-1) significantly restored medullary flow signals to normal. CBF and MAP were not altered whether H₂O₂ was infused alone or coinfused with catalase. H₂O₂ at infusion rates of 7.5 and 15 nmol · min^-1 · kg^-1 also decreased renal MBF by 5 and 20%, respectively (data not shown).

View larger version (22K): [in this window] [in a new window]   Fig. 6. Effects of renal medullary interstitial infusion (RI) of H2O2 and catalase on MAP and cortical and medullary blood flow. Values are means ± SE (n = 7). *P < 0.05 vs. control; #P < 0.05 vs. H2O2.

The effects of renal medullary interstitial infusion of H₂O₂ and catalase on renal excretory function are presented in Fig. 7. Medullary interstitial infusion of H₂O₂ at 30 nmol · min^-1 · kg^-1 produced a marked decrease in urine flow rate and Na⁺ excretion. Maximal reduction of urine flow rate and Na⁺ excretion was 50 and 47%, respectively. However, infusion of H₂O₂ into the renal medulla at 7.5 nmol · min^-1 · kg^-1 did not significantly alter urine flow rate and Na⁺ excretion (data not shown). In the presence of catalase (10 mg · min^-1 · kg^-1), infusion of H₂O₂, even at the highest dose used in the present study (30 nmol · min^-1 · kg^-1), had no effect on urine flow rate and Na⁺ excretion. In all these experiments, MAP, urine flow rate, and Na⁺ excretion in the contralateral kidney were not significantly altered.

View larger version (21K): [in this window] [in a new window]   Fig. 7. Effects of renal medullary interstitial infusion of H2O2 and catalase on renal function. Values are means ± SE (n = 7). *P < 0.05 vs. control; #P < 0.05 vs. H2O2 (30 nmol · min-1 · kg-1).

	DISCUSSION

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION DISCLOSURES REFERENCES

 
The present study determined the tissue levels of H₂O₂ in the renal cortex and medulla in Sprague-Dawley rats by in vivo microdialysis and microfluorometry using Amplex red assay, which identified the endogenous production of this reactive oxygen species in different kidney regions and provided guidance for choosing the doses of tempol and H₂O₂ for renal medullary infusion. Amplex red (N-acetyl-3,7-dihydroxyphenoxazine) is a highly sensitive and chemically stable fluorogenic probe that is used to quantitate H₂O₂. This indicator has been shown to be reliable with very high specificity (17, 30) and, recently, was used to detect H₂O₂ released from tissues or cells (26, 29) or generated in enzyme-coupled reactions (6, 19). By use of a microtiter plate reader, the reaction stoichiometry of Amplex red and H₂O₂ was determined to be 1:1, which could be used to detect as little as 10 pmol of H₂O₂ in a 100-µl volume (29). In previous studies, several fluorescent reagents have been used for the quantitation of H₂O₂. Scopoletin, a naturally occurring fluorescent compound, can be oxidized by H₂O₂ to a nonfluorescent product. Although it is extensively used for measurements of H₂O₂ production (4), scopoletin has a low extinction coefficient and short wavelength spectrum, which restricts its use in a wide range of different experiments (29). Compared with other fluorometric and spectrophotometric assays for the detection of H₂O₂, Amplex red has been found to be more sensitive to H₂O₂ with high selectivity, and there is very little spontaneous increase in Amplex red fluorescence with time (17). Furthermore, this oxidase-catalyzed assay using Amplex red results in an increase in fluorescence on oxidation, rather than a decrease in fluorescence, as in the scopoletin assay. As shown in Fig. 1, the high sensitivity and great linearity of the resorufin fluorescence intensity from the reaction of Amplex red with H₂O₂ suggest that this method could be used for the measurement of a wide range of H₂O₂ concentrations.

It is well known that H₂O₂ freely crosses biological membranes, and the rate of its production is closely related to O₂^-· and ·OOH (7). Therefore, the measurement of H₂O₂ has been often used to reflect oxidative status in the tissues or cells. In the present study, we detected H₂O₂ concentrations in interstitial microdialysates from the renal cortex and medulla. Because the dialysis efficiency of H₂O₂ across the membrane of the probe was 96% at a perfusion rate of 2 µl/min, measured H₂O₂ concentrations in the microdialysates largely represent its tissue concentrations in the inter-stitium. Interestingly, the basal level of H₂O₂ in the renal medulla was twofold higher than that in the renal cortex. This suggests that, under physiological conditions, the renal medulla is exposed to higher levels of oxidative stress than the cortex. These results are consistent with those obtained by detecting the production of O₂^-· (32). The present results also show that basal levels of H₂O₂ in the renal medulla exerted a moderate action on renal medullary basal vascular tone and renal excretory function. Reduction of basal renal medullary H₂O₂ levels by infusion of catalase only increased renal MBF by 10% and water and Na⁺ excretion by 12 and 16%, respectively.

Consistent with the findings reported previously, the present study suggests that O₂^-· is more importantly involved than H₂O₂ in the control of renal MBF and renal water and Na⁺ excretion. Tempol, an SOD mimetic of O₂^-·, increased MBF by 42% and water and Na⁺ excretion by 35 and 47%, respectively. In the presence of catalase, tempol-induced increases in renal MBF and renal water and Na⁺ excretion were markedly enhanced. The results indicate that H₂O₂ production by tempol may counteract the action of tempol. By microdialysis, we indeed found that tempol produced H₂O₂ when infused into the renal medulla and that exogenous catalase infusion blocked this tempol-induced H₂O₂ production. It seems that although tempol largely blocks the detrimental effects of O₂^-· in the renal medulla, H₂O₂ production during dismutation of O₂^-· may limit its beneficial antioxidant action. This counteracting action of H₂O₂ on tempol-induced renal medullary vasodilation and natriuresis may be one of the important reasons for the failure to prevent hypertension induced by exaggerated oxidative stress in the renal medulla, as reported in our previous study (14). In that study, it was found that chronic infusion of tempol into the renal medulla could not prevent the development of hypertension induced by SOD inhibition. In the presence of exogenous catalase, however, chronic infusion of tempol effectively prevented hypertension. Taken together, these results indicate that tempol as an antioxidant dilates renal medullary vessels, increases MBF, and enhances renal water and Na⁺ excretion, thereby producing an antihypertensive effect. These effects may represent the important therapeutic basis for the prevention or treatment of some forms of hypertension. However, because tempol produces H₂O₂ during dismutation of O₂^-·, especially when its concentrations are high in tissues such as the renal medulla because of local infusion or exaggerated oxidative stress, it may not be very effective in preventing hypertension associated with exaggerated oxidative stress.

The present findings do not imply that the antihypertensive effects of tempol observed by others in various models of hypertension were due to lack of H₂O₂ production. There is no doubt that tempol could react with O₂^-· to produce H₂O₂, but it seems that the hypertensive effect of H₂O₂ was not exhibited in those studies (2, 15, 25, 27). It is most likely that tissue H₂O₂ levels, especially those in the renal medulla, were probably lower in previous experiments than in the present study. First, the local delivery of tempol into the renal medulla produced high concentrations of H₂O₂ in this region, which counteracted its renal antihypertensive action, as shown in our chronic experiments (13). In previous studies where tempol was administered orally or intravenously, tempol could be converted to other active components through the liver or other systems, or tempol-induced H₂O₂ could be metabolized systemically. Second, in the present study, tempol was administrated to simulate a condition with an exaggerated local oxidative stress induced by an SOD inhibitor, diethyldithiocarbamic acid (14). Under this circumstance, large amounts of H₂O₂ could be produced by infusion of a high dose of tempol or achieved by direct infusion of H₂O₂. In previous studies, however, tempol was administered to hypertensive animals such as spontaneously hypertensive or Dahl salt-sensitive rats to simply determine whether it prevents hypertension. It is likely that the degree of renal medullary oxidative stress in those rats does not achieve the levels seen with the direct administration of SOD inhibitors. The results of the present studies, therefore, indicate that, especially in forms of hypertension with exaggerated renal oxidative stress, tempol should be used with caution.

Previous studies have reported that high levels of H₂O₂ are cytotoxic through its oxidant effect. It is therefore thought that H₂O₂ as an oxygen reactive species must be rapidly eliminated from tissues and cells. Although H₂O₂ was also reported to be increased in patients with hypertension, chronic renal failure, and other diseases (12), the detrimental effects of H₂O₂ in the kidney have not been studied. The present study examined whether H₂O₂ has direct effects to produce renal dysfunction. It was found that direct delivery of H₂O₂ into the renal medulla significantly increased the concentration of H₂O₂ in this kidney region and largely decreased MBF and water and Na⁺ excretion. These results suggest that excessive H₂O₂ in the renal medulla produces vasoconstriction and antinatriuresis. Given the importance of renal MBF and Na⁺ excretion in the development of hypertension, elevations of H₂O₂ in the region could contribute to medullary vasoconstriction and Na⁺ retention, thereby contributing to the development of hypertension.

In summary, the present study found that H₂O₂ was detectable in the renal tissue in vivo using microdialysis. Tempol-induced H₂O₂ production was found to counteract the vasodilator or natriuretic actions of this SOD mimetic. Increased H₂O₂ directly constricted medullary vessels and decreased Na⁺ excretion. We concluded that the increase of H₂O₂ in the renal medulla may result in the development of hypertension. Because of its H₂O₂-producing action, tempol must be used with caution as an antihypertensive compound in forms of hypertension with exaggerated oxidative stress.

	DISCLOSURES

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION DISCLOSURES REFERENCES

 
This study was supported by National Institutes of Health Grants HL-29587 and DK-54927.

	FOOTNOTES

 

Address for reprint requests and other correspondence: A.-P. Zou, Dept. of Physiology, Medical College of Wisconsin, 8701 Watertown Plank Rd., Milwaukee, WI 53226 (E-mail: azou{at}mcw.edu).

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.

	REFERENCES

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION DISCLOSURES REFERENCES

 

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