INTRODUCTION

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THERMONEUTRAL WATER IMMERSION (WI) to the neck in humans induces redistribution of blood from the caudal to the cephalad parts of the body and movement of fluid from the interstitial to the intravascular space. Therefore, central and total blood volume is expanded, which is accompanied by a natriuresis and a diuresis. The generally accepted hypothesis is that the natriuresis and diuresis of WI is initiated by stimulation of cardiopulmonary volume receptors (14). This hypothesis is, however, too simplistic, because we (25) have previously observed that the decrease in plasma colloid osmotic pressure and/or increase in plasma volume per se also might play a role for the initiation of the natriuresis. The natriuresis and diuresis of WI are probably multifactorial in origin and comprise an interaction of cardiovascular, neural, physical, and humoral factors. The quantitative contribution of each of the efferent components is still not defined.

To investigate the qualitative contribution of the renin-angiotensin system to the natriuresis of WI, Epstein and Saruta (16) observed that plasma renin activity and aldosterone were suppressed with very similar temporal profiles. In a later study in anephric humans, Epstein et al. (15) showed that plasma aldosterone was not suppressed by WI. In addition, we (21) have in a recent study shown that plasma ANG II is suppressed by WI. Therefore, results of these studies strongly indicate that suppression of the renin-angiotensin-aldosterone axis is an important mechanism of the natriuresis of WI in humans.

In the present study we tested the hypothesis that suppression of generation of ANG II is a mechanism of the natriuresis of WI in humans. ANG II was intravenously infused to prevent suppression of plasma ANG II by WI, and the effect on the natriuretic response was simultaneously monitored.

In a second protocol, ANG II was infused intravenously in two different amounts on two separate study days during WI to delineate the tubular site(s) of action of ANG II on renal sodium handling by the lithium clearance (C_Li) method. The two dosages were used because we at the time of study did not know whether the low level would have any tubular effect.

	MATERIALS AND METHODS

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Studies were carried out in healthy young males. All had a negative history of cardiovascular and kidney diseases and exhibited normal values of routine clinical examinations. All subjects had their urine tested for protein, erythrocytes, and glucose. All tests were negative. All subjects denied taking any medication at the time of the study. The experimental protocols were approved by the Ethics Committee of Copenhagen (V.200.2088/91; KF12-145/99), and after careful oral and written explanation, written consent was obtained according to the Declaration of Helsinki. The experiment fully conforms to the Guiding Principles for Research Involving Animals and Human Beings of the American Physiological Society. The experiment consisted of two almost identical protocols (protocols 1 and 2).

Protocol 1

Each subject was investigated in the upright seated posture during three interventions on different study days with the sequence in a randomized, balanced order between the subjects and separated by at least 4 wk. The sessions consisted of 1) WI to the neck for 3 h with simultaneous infusion of vehicle (WI + placebo), 2) WI to the neck for 3 h with simultaneous low-dose ANG II infusion of 0.5 ng · kg body wt¹ · min¹ (WI + ANG II-low), and 3) a seated time control for 3 h in an empty tank with simultaneous infusion of vehicle (Con). Each session was preceded and followed by the subject being seated outside the water for 1.5 and 1 h, respectively.

For 4 days before each experimental day, the subject was provided with food containing a fixed content of sodium (135-150 mmol/24 h). Twenty-four-hour urine collections were made during the final 2 days of each dietary period. Water intake was ad libitum. No food or fluid intake was allowed for 12 h before the experiment.

From 10:00 PM the evening before the experiment, the subject was confined to the laboratory. He was awakened at 7:15 AM and weighed. A short 18-gauge venous catheter (Venflon, Viggo-Spectramed) was inserted into each cubital vein: one for collection of blood and one for infusion of vehicle and/or ANG II. After emptying the bladder, the subjects drank 400 ml of tap water and were seated (wearing a bathing suit) in a chair. Thereafter, they were subjected to WI or Con. At all times during the experiment (before, during, and after immersion or control), both of the subject's arms were kept resting on a support above the water and always at the same distance above the heart. Arterial pressures were corrected for hydrostatic errors by adding to the recorded pressures the distance from the cuff to the fourth intercostal space divided by 1.36.

WI was performed by lowering the subject by a hoist into an insulated plastic tank, which was empty during Con or filled with tap water during WI. During the pre- and postimmersion periods, the subject sat in the chair above the water. Average water temperature varied over time between 34.5 ± 0.02 and 34.7 ± 0.07°C, room temperature between 25.8 ± 0.02 and 26.2 ± 0.06°C, and relative air humidity between 30.3 ± 1.9 and 44.8 ± 2.07%.

Arterial pressures and heart rate (HR) were determined at half-hourly intervals and cardiac output (CO) and left atrial diameter every hour. A total of 300 ml of blood was collected during the experiment according to the time intervals indicated in Fig. 1 and Table 1. Before each blood sampling, 2 ml of blood were drawn to empty dead space. After each sampling of blood, the catheter was flushed with an amount of isotonic saline equal to that of the collected blood. Finally, at hourly intervals the subjects stood briefly on a support to empty the bladder and thereafter drank 200 ml of tap water. Measurements and procedures were always performed in the following sequence: blood sampling, arterial pressures, left atrial diameter, HR, CO, urine collection, and determination of residual urine by ultrasound.

View larger version (24K): [in this window] [in a new window]   Fig. 1.   Protocol 1: renal sodium excretion (UNaV; A), plasma concentration of ANG II (B), plasma concentration of aldosterone (Aldo; C), and mean arterial pressure (MAP; D) before, during, and after 3 h of water immersion (WI + placebo; ), water immersion and infusion of 0.5 ng ANG II · kg1 · min1 (WI + ANG II-low; ), and a seated time control (Con; ). Values are means ± SE of n = 8. * Significant difference compared with preimmersion value. # Significant difference from other 2 sessions at same experimental point in time. + Significant difference from Con at same experimental point in time.

ANG II (Clinalfa, Switzerland) infusion started simultaneously with WI. Subjects received a 3-h intravenous infusion of either ANG II at 0.5 ng · kg¹ · min¹ in 0.9% saline or vehicle (0.9% saline). A 50-ml syringe pump (Braun) delivered the infusion at a rate of 3-4 ml/h. The experiment was performed in a single-blinded fashion.

Plasma concentrations of norepinephrine (NE) and epinephrine (Epi) were measured with a radioenzymatic assay (9). Plasma concentrations of ANG II were measured according to Bie and Sandgaard (4). Plasma aldosterone was measured by radioimmunoassay with a commercially available kit (Coat-A-Count, DPC), and plasma concentration of atrial natriuretic peptide (ANP) was measured by radioimmunoassay (41).

Plasma protein concentration (P_prot) was measured in duplicate in a refractometer (pocket refractometer, Bellingham & Stanley). Concentrations of Na⁺ and K⁺ in urine and plasma were measured in fresh samples with an ion-selective electrode system (KNA-2, Radiometer, Copenhagen, Denmark).

Echocardiographic recordings (model SSD 500; Aloka, Japan) of left atrial diameter were obtained using the parasternal long-axis view in M-mode according to the criteria of Feigenbaum (17). Left atrial diameter was determined from the average of three M-mode pictures, which in a blinded fashion were analyzed by the same investigator with regard to all of the subjects.

HR was calculated from electrocardiogram recordings. Systolic, diastolic, and mean arterial pressures (MAP) were measured every half hour in the brachial artery by oscillometry (Propaq 102, Protocol Systems, Beaverton). CO was estimated with a noninvasive inert gas rebreathing technique (AMIS 2001; Innovision, Odense, Denmark) as previously described in detail (6, 10). Total peripheral vascular resistance (TPR) was calculated by dividing MAP by CO.

Residual urine was calculated by the formula described by Roehrborn and Peters (39). Urine volumes were corrected if calculated residual urine exceeded 30 ml. Urine flow rate (V) and renal sodium excretion (U_NaV) were calculated by conventional formulas.

Protocol 2

1

1

1

1

All procedures were the same as in protocol 1, except as follows. 1) LiCO₃ (12.15 mmol; 450 mg) was administered to the subjects at 10:00 PM on the evening before the experiment for determination of lithium clearance. 2) Plasma concentrations of ANG II, aldosterone (DSL-8600, obtained from Diagnostic Systems Laboratories, Webster, TX), NE, and Epi were measured by other assays (3, 26). 3) Glomerular filtration rate (GFR) was determined by renal clearance of ⁵¹CR-EDTA (Amersham, UK) (7), and plasma and urinary lithium concentrations were determined by atomic absorption spectrophotometry (Perkin Elmer 1100 B, Norwalk, CT) (1). 4) Echocardiography of the left atrium was replaced by central venous pressure measurement. It was measured through a fluid-filled catheter inserted from a cubital vein to the intrathoracic region. 5) Blood was sampled from the central venous catheter. 6) In addition to the infusion of 0.5 ng · kg¹ · min¹, ANG II was also infused at a rate of 1.5 ng · kg¹ · min¹ (WI + ANG II-high).

Renal sodium clearance (C_Na) and C_Li were calculated as the ratio between the urinary excretion rates and the mean plasma concentrations. The absolute proximal tubular reabsorption rate of fluid (APR_Fluid) was determined as GFR  C_Li. The absolute proximal tubular reabsorption rate of sodium (APR_Na) was determined as (GFR  C_Li) × P_Na, where P_Na is plasma concentration of Na. Absolute distal reabsorption rate of sodium (ADR_Na) was calculated as (C_Li  C_Na) × P_Na, and fractional distal sodium reabsorption (FDR_Na) was calculated as (1  C_Na/C_Li). Whole kidney fractional excretion of lithium (FE_Li) and sodium (FE_Na) were determined as C_Li/GFR and C_Na/GFR, respectively.

Statistics

	RESULTS

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Protocol 1

Renal variables. Infusion of ANG II attenuated the natriuresis of WI (Fig. 1) because during WI + placebo, U_NaV increased from 87 ± 16 µmol/min to a peak of 262 ± 14 µmol/min during the third hour of immersion (P < 0.05), whereas U_NaV only increased from 73 ± 8 µmol/min to a peak of 160 ± 30 µmol/min (P < 0.05) during WI + ANG II-low. Cumulative sodium excretion during WI + placebo was significantly different from cumulative sodium excretion during WI + ANG II-low during the 3 h of immersion (39 ± 3 vs. 23 ± 4 mmol/180 min; P < 0.05; paired t-test). Values during Con varied insignificantly between 75 ± 12 and 58 ± 7 µmol/min. Urine volumes were corrected five times for residual volumes.

Plasma hormones. Plasma concentration of ANG II (Fig. 1) decreased from 12 ± 2 to 4 ± 1 pg/ml during all of the 3 h of WI + placebo (P < 0.05). During WI + ANG II-low, plasma ANG II was prevented from decreasing. During Con, plasma ANG II increased significantly from 8 ± 2 to 16 ± 3 pg/ml (P < 0.05).

Plasma proteins and electrolytes. WI + placebo and WI + ANG II-low suppressed plasma proteins significantly throughout the immersion period (Table 1). Plasma proteins did not change during Con. During Con, plasma sodium varied insignificantly between 138.4 ± 0.4 and 139.3 ± 0.3 mmol/l, and during WI + ANG II-low, plasma sodium varied insignificantly between 138.4 ± 0.5 and 138.8 ± 0.4 mmol/l. During WI + placebo, plasma sodium increased from 138.8 ± 0.4 to 140.1 ± 0.4 mmol/l (P < 0.05). Plasma potassium decreased during WI + placebo from 4.3 ± 0.1 to 4.0 ± 0.0 mmol/l (P < 0.05). During Con and WI + ANG II-low, plasma potassium varied insignificantly between 4.0 ± 0.0 and 4.2 ± 0.1 mmol/l and between 3.9 ± 0.1 and 4.1 ± 0.1 ml/min, respectively.

Cardiovascular variables. MAP did not change during Con and WI + placebo (Fig. 1) but increased during WI + ANG II-low from 87 ± 2 to 94 ± 2 mmHg during the second and third hours (P < 0.05). CO also increased and TPR decreased during WI + placebo and WI + ANG II-low (Table 2, P < 0.05). CO and TPR were unchanged during Con.

Protocol 2

Renal variables. U_NaV exhibited the same response to WI + placebo, WI + ANG II-low, and Con as in protocol 1 (Fig. 2). During WI + ANG II-high, the natriuresis was abolished (Fig. 2). The temporal profile of C_Na and FE_Na (Table 3) followed that of U_NaV as indicated in Fig. 2. GFR did not change significantly during any session (Table 3). Urine volumes were corrected six times for residual volumes.

View larger version (26K): [in this window] [in a new window]   Fig. 2.   Protocol 2: renal UNaV (A), plasma concentration of ANG II (B), lithium clearance (CLi; C), and fractional distal reabsorption of sodium (FDRNa; D) before, during, and after 3 h of WI + placebo (), WI + ANG II-low (), WI and infusion of 1.5 ng ANG II · kg1 · min1 (WI + ANG II-high; ), and Con (). Values are means ± SE of 10 subjects during Con (CLi and FDRNa, n = 8), 10 subjects during WI + placebo (CLi and FDRNa, n = 8), 7 subjects during WI + ANG II-low (CLi and FDRNa, n = 5), and 8 subjects during WI + ANG II-high (CLi and FDRNa, n = 7). * Significant difference compared with preimmersion value.

Plasma hormones, plasma proteins and electrolytes, and cardiovascular variables. As depicted in Fig. 2 and Tables 1-3, the endocrine and cardiovascular responses were very similar to that of protocol 1. It should be noted that ANG II during WI + ANG II-low increased slightly from 18 ± 4 to 35 ± 8 pg/ml (P < 0.05) and increased from 18 ± 2 to 57 ± 10 pg/ml (P < 0.05) during WI + ANG II-high. Values not shown exhibited the same response as in protocol 1, and WI + ANG II-low and WI + ANG II-high did not differ.

Protocols 1 and 2

1

1

View larger version (26K): [in this window] [in a new window]   Fig. 3.   Protocols 1 and 2: renal UNaV (A) and plasma concentration of ANG II (B) before, during, and after 3 h of WI + placebo (), WI + ANG II-low (), and Con (). Values are means ± SE of n = 15. * Significant difference compared with preimmersion value. # Significant difference from other 2 sessions in same experimental point in time.

U_NaV before immersion and during Con, WI, and WI + ANG II-low was higher in protocol 2 (lithium pretreatment) than in protocol 1 (P < 0.05, unpaired t-tests).

	DISCUSSION

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Our findings demonstrate that when a decrease in plasma concentration of ANG II is prevented, the natriuretic response to WI is attenuated. Therefore, suppression of generation of ANG II is a mechanism of the natriuresis of WI in humans. Furthermore, infusion of ANG II prevented an increase in the end-proximal delivery of tubular fluid, which was otherwise induced by WI, and facilitated the fractional distal reabsorption of sodium, probably via an effect on aldosterone release.

WI-Induced Volume Stimulus

ANG II Clamping

In protocol 1, the level of plasma ANG II during WI + ANG II-low was below the level of Con (Fig. 1), whereas it was slightly above that of Con in protocol 2 (Fig. 2). Despite these under- and overshootings, the natriuresis was attenuated to a similar extent (56 ± 15 vs. 47 ± 10%). Therefore, these variations in plasma concentrations of ANG II, when WI + ANG II-low and Con of the two protocols were compared, were too small to induce different effects on the kidneys. The different levels, however, of plasma ANG II may theoretically have caused an under- or overestimation, respectively, of the importance of ANG II on the natriuretic response to WI. The combined results, however, indicate that the natriuresis was blunted by 52 ± 13% when plasma ANG II was clamped to the level of Con (Fig. 3).

Plasma ANG II , MAP, and FE_Na

Intrarenal Mechanisms of ANG II

To delineate the tubular site(s) of action of ANG II on renal sodium handling, we employed the C_Li method. This method relies on the assumption that C_Li is a quantitative measure of end-proximal fluid delivery to the thin descending limb of loop of Henle (27, 31). We observed that the natriuresis of WI + placebo was accompanied by a significant increase in C_Li during the second hour and that low- and high-dose infusion of ANG II (Fig. 2) prevented the increase in C_Li. An increase in C_Li during WI and a decrease during ANG II infusion have previously been reported (13, 36, 38). A change in C_Li can be explained by a change in GFR, a true change in APR_Fluid, or both. We were not able to detect any changes in either GFR or calculated APR_Fluid during WI + placebo, WI + ANG II-low, and WI + ANG II-high (Table 3). Therefore, the mechanism(s) behind the changes in C_Li cannot be deduced from our results. Results of previous experiments, however, suggest that GFR and C_Li increase in parallel during immersion (36) and that they decrease during ANG II infusion (13, 38). This indicates that there is an effect of ANG II on the renal vasculature but that there is no effect of ANG II on the proximal tubular epithelium (44).

The proximal reabsorption of fluid and sodium are mainly load independent (44). Therefore, changes in APR_Fluid and APR_Na may reflect changes in proximal tubular reabsorption. In the present study we did not observe any evidence of a direct effect of ANG II on proximal tubular reabsorption of sodium as demonstrated by an unchanged APR_Na (Table 3). This is in accordance with previous results in humans (13, 38). It is, however, well accepted that ANG II exerts its primary effects on the proximal tubular epithelium (19, 24). Therefore, the lack of change in calculated APR_Na during suppression of generation of endogenous plasma ANG II and during ANG II infusion could reflect undetectable changes in APR_Na due to variations in the GFR and C_Li measurements. It is, however, likely that unchanged transport effects of ANG II on proximal luminal receptors during WI + placebo, WI + ANG II-low, and WI + ANG II-high can explain the unchanged APR_Na (30). Boer et al. (5) have demonstrated that proximal intraluminal concentrations of ANG II was unchanged in volume expanded rats, and Quan and Baum (34) have demonstrated that addition of ANG II to proximal tubular fluid did not enhance the proximal reabsorption rate. In contrast, application of angiotensin-converting inhibitors in humans and rats decreased the proximal reabsorption rate (22, 34). Therefore, unchanged transport effects of ANG II on proximal luminal receptors may explain the unchanged APR_Na in the present study.

The tubular reabsorption of sodium and water is mainly load independent, but some load dependence cannot be excluded. Therefore, changes in FE_Li may indicate an effect on the proximal tubular epithelium. We are, however, of the opinion that APR_Na and APR_Fluid are the best suited to reflect biological effects in the proximal tubular epithelium. FE_Li increased during WI + placebo (Table 3). This was prevented by ANG II infusion (Table 3). The increase during immersion and the decrease during ANG II infusion in FE_Li are in accordance with results of previous experiments (11, 13, 32, 35-38). Thus the prevention of an increase in end-proximal fluid delivery and the prevention of an increase in FE_Li by ANG II infusion during immersion could indicate an effect of ANG II on proximal nephron sodium balance during WI.

In the integrated distal segments of the nephron, we observed that FDR_Na decreased in response to immersion (Fig. 2) but that ADR_Na was unchanged (Table 3). A decrease in the FDR_Na suggests a decrease in distal reabsorption of sodium due to the load-dependent sodium reabsorption in these nephron segments (48). Infusion of ANG II affected FDR_Na in a dose-dependent manner (Fig. 2). Our results are in compliance with previous results of Rabelink et al. (36) who observed a decrease in FDR_Na during immersion. Furthermore, FDR_Na increases during infusion of ANG II in humans (13, 38). Our data do not allow any firm conclusion based on the statistics on the effect of ANG II on aldosterone release in protocol 2 (Table 1). However, it still remains a possibility that the low level of ANG II infusion attenuated the suppression of aldosterone release, which could have constituted a mechanism of the augmented FDR_Na. It is also a possibility that ANG II per se directly affected the distal tubules and thus FDR_Na (47).

Our results suggest that the natriuresis of WI in humans depends on an increase in end-proximal fluid delivery and a simultaneous decrease in FDR_Na. It is conceivable that end-proximal fluid delivery is regulated by ANG II and that it modulates FDR_Na through an effect on aldosterone release (29).

Lithium and Renal Sodium Excretion

Conclusions

Perspectives

Our data also indicate that at least part of the antinatriuretic effect of ANG II is mediated by an increase in distal reabsorption of sodium. Whether this is a direct effect of ANG II on the distal epithelium or whether it is mediated by an effect through aldosterone release should be investigated, e.g., by ANG II infusion in subjects pretreated with spironolactone.

Finally, the results of this study are also of relevance for understanding pathophysiology of heart disease. Gabrielsen et al. (18) have recently shown that when plasma ANG II is high in heart failure patients, the natriuresis of WI is attenuated. By treating the patients with an angiotensin-converting enzyme inhibitor, the natriuresis of WI was restored to that of normal. Thus WI in combination with modulation of plasma ANG II might be applicable for future studies on mechanisms of disease with fluid volume derangements.