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1 Departments of Pediatrics and 2 Internal Medicine, University of Texas Southwestern Medical Center at Dallas, Dallas, Texas 75235-9063
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ABSTRACT |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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In the present study, we examined whether the effect of
endogenously produced angiotensin II on proximal tubule transport in
the male Sprague-Dawley rat is regulated by acute changes in extracellular volume. We measured the magnitude of endogenous angiotensin II-mediated stimulation of transport by sequentially perfusing proximal tubules in vivo, first with an ultrafiltrate-like solution, then by reperfusion of the same tubule with an
ultrafiltrate-like solution containing
10
8 M losartan (angiotensin
II receptor antagonist). During volume contraction,
108 M losartan decreased
volume reabsorption from 4.20 ± 0.50 to 1.70 ± 0.30 nl · mm1 · min1
(P < 0.05), a decrease of 58.0 ± 7.0%. In contrast, after acute volume expansion,
108 M losartan decreased
volume reabsorption from 1.84 ± 0.20 to 1.31 ± 0.20 nl · mm1 · min1
(P < 0.05), a decrease of 29.6 ± 9.0%. In hydropenic rats, addition of exogenous luminal angiotensin II
had no effect on transport. However, in volume-expanded rats, addition
of 108 M angiotensin II
increased volume reabsorption from 2.10 ± 0.34 to 4.38 ± 0.59 nl · mm1 · min1
(P < 0.005). These data are
consistent with endogenously produced angiotensin II augmenting
proximal tubule transport to a greater degree during volume contraction
than after volume expansion.
autocrine; losartan; microperfusion; kidney
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INTRODUCTION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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THE RENAL PROXIMAL TUBULE can synthesize and secrete angiotensin II into the lumen (4, 5, 25, 27). Components of the renin-angiotensin system found within the proximal tubule include angiotensinogen and its mRNA, renin activity in lysates of proximal tubule cells in primary culture, and renin mRNA detected in proximal tubule cells in primary culture by reverse transcription and polymerase chain reaction (13, 20, 21, 24, 29). Angiotensin-converting enzyme activity has been localized to the luminal brush-border membrane, and receptors for angiotensin II have been found on both the basolateral and luminal membranes (6, 7, 9, 10, 29). Angiotensin II has been detected in native tubular fluid and in rat proximal tubules perfused with an artificial tubular fluid at concentrations ranging from 100- to 1,000-fold higher than in plasma (4, 5, 27).
Using in vivo microperfusion, we have recently shown that endogenously
produced and luminally secreted angiotensin II modulates proximal
tubule transport in the hydropenic rat (23). Luminal perfusion of
108 M losartan (angiotensin
II receptor antagonist) or
104 M enalaprilat
(angiotensin-converting enzyme inhibitor) decreases the rate of
proximal tubule transport by 35-40% (23). The decrease in
transport observed with enalaprilat was completely reversed with
addition of exogenous 1011
or 108 M luminal
angiotensin II (23). These observations are consistent with endogenous
angiotensin II stimulating proximal tubule transport in an autocrine or
paracrine fashion.
The aim of this study was to examine whether the effect of endogenously produced and luminally secreted angiotensin II on proximal tubule volume reabsorption is regulated by acute changes in extracellular volume. The magnitude of the reduction in proximal tubule transport observed after addition of luminal losartan was used as a measure of the magnitude of the effect of angiotensin II on proximal tubule transport.
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METHODS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Preparation of animals. Male
Sprague-Dawley rats weighing between 180 and 240 g were used for this
study. Rat preparation and the in vivo microperfusion procedure
described below have been previously described in detail (16, 17, 23).
Briefly, all animals were allowed free access to food and water before anesthesia with intraperitoneal Inactin (100 mg/kg). Rats were placed
on a servo-controlled heated table set to maintain body temperature at
37°C. The jugular vein was cannulated for infusion of normal saline
at 2.8 ml/h. A flank incision was used to expose the left kidney, which
was then immobilized in a Lucite cup. The kidney was bathed with
water-equilibrated light mineral oil heated to 37°C that was
previously bubbled with 95%
O2-5%
CO2. The ureter was cannulated
with polyethylene tubing to ensure free flow of urine. After
microperfusion experiments during the hydropenic period were completed,
the rat was volume expanded with normal saline and a normal saline
solution containing 5% bovine serum albumin (1, 12). Normal saline was
infused at a volume equal to 10% body weight over 1 h (~20
ml/h), followed by 3% body wt/h (~6 ml/h) (1). The 5%
bovine serum albumin solution contained 140 mM NaCl and 4 mM KCl and
was infused at 1 ml/100 g weight over 45 min (~2 ml/45 min), followed
by 0.15 ml · 100 g
wt1 · h1
(~0.3 ml/h) (12). Serial hematocrits were obtained at the time of
vessel cannulation (prior to further surgery), 1 h after all surgery
had been completed, and 1 h after volume expansion had been completed.
Micropuncture surgery has previously been shown to reduce plasma volume
and raise serial hematocrits (18, 23). As seen in Table
1, hematocrits and plasma angiotensin II
levels rose with volume contraction and fell to presurgical levels
following volume expansion (P < 0.001). Conversely, urine flow rate and urinary sodium excretion were
low during volume contraction and rose significantly with volume
expansion. Using a very similar volume expansion protocol, Braam et al.
(5) demonstrated a similar fall in hematocrit and a rise in plasma
angiotensin II levels, mean arterial pressure, urinary flow rate, and
urinary sodium excretion, as well as fractional excretion of sodium.
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In vivo microperfusion. Proximal tubule segments on the surface of the kidney were initially mapped with an injection of a small droplet of oil, and early and late loops were identified. A wax block was inserted into the lumen of an early loop by a hydraulic Microdrive (Trent Wells, Coulterville, CA), which prevented any native glomerular ultrafiltrate from flowing into the tubule segments distal to the block. The wax block also prevented the native glomerular ultrafiltrate from escaping the tubule lumen and thus likely raised the hydrostatic pressure in Bowman's space and stopped ongoing single-nephron glomerular filtration. Subsequently, a microperfusion pipette was inserted into the lumen immediately distal to the wax block, and an ultrafiltrate-like solution was perfused at 30 nl/min. Microperfusion was accomplished using a microperfusion pump system (K. Effenberger; Vestavia Scientific, Birmingham, AL). In a late proximal tubule loop distal to the perfusion pipette, a collection pipette was inserted, and the perfused ultrafiltrate-like solution was collected after an oil block was placed distally. Fluid collections were made over a 2- to 3-min period. The length of the tubule between the perfusion and collection sites averaged 2.6 ± 0.2 mm. The composition of the ultrafiltrate-like solution was (in mM) 120 NaCl, 25 NaHCO3, 5 KCl, 1 MgSO4, 1.8 CaCl2, 1 Na2PO4, 5 glucose, 5 alanine, 5 urea, and FD & C green dye no. 3. Exhaustively dialyzed [methoxy-3H]inulin was added as a volume marker.
To examine the effect of
108 M losartan (angiotensin
II receptor antagonist; DuPont, Wilmington, DE) on proximal tubule
transport, each proximal tubule was perfused twice, first with the
control ultrafiltrate-like solution, followed by a second perfusion
with the same ultrafiltrate-like solution containing
108 M losartan (30). Both
initial and subsequent tubule perfusions and fluid collections were
made from the same tubule puncture sites, thus allowing paired data to
be obtained. The "double micropuncture" technique was performed
in both volume-contracted and volume-expanded animals. Luminally
perfused losartan acts primarily on the luminal brush border receptors.
It is unknown whether losartan can traverse the proximal tubule cell
and act on the basolateral angiotensin II receptors. However, luminal
losartan has been shown to inhibit volume reabsorption and bicarbonate
transport in rabbit proximal convoluted tubules perfused in vitro in
the absence of bath angiotensin II (2).
We next examined the effect of luminal angiotensin II on proximal
tubule transport in the volume-expanded animals with luminal perfusion
of exogenous angiotensin II at
106,
108, and
1010 M
([Asn1,Val5]angiotensin
II; Sigma Chemical, St. Louis, MO). In vivo microperfusion of the
volume-expanded animals began 1 h after volume expansion had been
completed.
After all collections were performed, the entire tubule was injected with liquid Microfil (Flow-Tech, Carver, MA) and allowed to harden overnight in the refrigerator. The kidney was later placed in 6 N HCl at 37°C for 1 h. The Microfil tubule casts were dissected and photographed, and the tubular length between the perfusion and collection sites was measured.
Plasma angiotensin II assay. Plasma
samples were collected 1 h after completion of animal surgery, during
volume contraction, and 1 h after volume expansion was completed.
Plasma samples were extracted on a phenyl-bonded sodium
phosphate-EDTA column (Bond-Elut; Analytichem, Harbor
City, CA). Prior to sample application, the column was prewashed with 3 ml of 90% methanol in water and 6 ml of distilled deionized water.
After the sample was applied, the column was then washed with 3 ml of
distilled deionized water, followed by 1.5 ml hexane, and finally 1.5 ml chloroform. The angiotensin peptides retained on the column were
then eluted with 2 ml of 90% methanol in water, dried under vacuum in
a Speed Vac, and subsequently stored at 
80°C until assay.
The angiotensin II assay was performed with an enzyme immunoassay kit (Peninsula Laboratories, Belmont, CA). Briefly, samples and standards are added to microtiter wells containing antibody to angiotensin II bound to the walls of the well. Next, biotinylated "tracer angiotensin II" is added to the well, which competes with angiotensin II in the sample or standard for binding to the angiotensin II antibody. The amount of biotinylated angiotensin II bound to the angiotensin II antibody is inversely proportional to the amount of angiotensin II in the sample. After incubation, avidin-horseradish peroxidase conjugate is added, which binds only to biotinylated angiotensin II. In the last step, a colorimetric agent (3,3',5,5'-tetramethyl benzidine dihydrochloride) is added to each well and allowed to react with bound horseradish peroxidase. The intensity of color depends on the amount of horseradish peroxidase bound to biotinylated angiotensin II. All microtiter wells are read in a colorimetric microtiter plate reader (Titertek Multiscan, McLean, VA), a standard curve is constructed from the optical density readings, and sample angiotensin II concentrations are read from this curve. A standard curve is constructed each time the assay was performed.
Analysis. All collected tubular fluid was transferred to constant-bore capillary tubing for measurement of volume with a micrometer (Mitutoyo, City of Industry, CA) and then mixed with scintillation fluid for radioactivity counting. The rate of fluid reabsorption was calculated as the difference between perfused and collected volumes divided by the time of collection divided by the tubule length. One tubule per rat was used for micropuncture. Thus, n represents the number of tubules and rats. Analysis of variance and Student's t-tests (paired and unpaired) were used to determine statistical significance. The post hoc test used following analysis of variance included the Student-Newman-Keuls multiple comparisons test. All data are expressed as means ± SE.
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RESULTS |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Effect of luminal losartan on proximal
tubule transport during volume contraction and volume
expansion. These studies were performed to investigate
the effect of losartan, an angiotensin II receptor antagonist, on the
proximal tubule volume reabsorptive rate during volume contraction and
volume expansion. As seen in Fig. 1,
administration of luminal
108 M losartan
significantly inhibited the rate of volume reabsorption by the proximal
tubule during volume contraction (4.2 ± 0.50 vs. 1.70 ± 0.30 nl · mm1 · min1,
P < 0.05). In contrast, after acute
volume expansion, administration of luminal
108 M losartan decreased
volume reabsorption to a far lesser degree (1.84 ± 0.20 vs. 1.31 ± 0.20 nl · mm1 · min1,
P < 0.05). Time controls performed
in the volume-expanded rats demonstrated no change in volume
reabsorption rates between the first and second perfusions (2.22 ± 0.78 vs. 2.13 ± 0.81 nl · mm1 · min1).
As seen in Fig. 2, the absolute and percent
decrement in proximal tubule transport resulting from the
administration of luminal 108 M losartan was
significantly greater during volume contraction (58 ± 7.0%) than
after volume expansion (29.6 ± 9.0%,
P < 0.05).
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Effect of luminal angiotensin II on proximal tubule
transport during volume expansion. These studies were
conducted to investigate the effect of
106,
108, and
1010 M luminal angiotensin
II on proximal tubule volume reabsorption in the acutely
volume-expanded rat. We and others have previously shown that
administration of 106,
108, and
1011 M luminal angiotensin
II in the volume-contracted rat had little or no effect on proximal
tubule transport (11, 17, 23). As shown in Fig.
3,
108 M luminal angiotensin
II increased proximal tubule volume reabsorption in the volume-expanded
rat from 2.10 ± 0.34 to 4.38 ± 0.59 nl · mm1 · min1
(P < 0.005). This rate of
proximal tubule volume absorption was comparable to that observed in
volume-contracted rats. In contrast, the rates of proximal tubule
volume reabsorption observed with 106 and
1010 M luminal angiotensin
II (2.22 ± 0.29 and 1.97 ± 0.20 nl · mm1 · min1,
respectively) were unchanged, compared with that observed in the
volume-expanded control (2.10 ± 0.34 nl · mm1 · min1).
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DISCUSSION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Angiotensin II has long been known to directly affect proximal tubule transport independent of changes in the glomerular filtration rate (3, 11, 14, 16, 17, 26). Physiological doses of angiotensin II stimulate proximal tubule transport in the absence of changes in glomerular hemodynamics or blood pressure (3, 11, 14, 16, 17). Using in vitro and in vivo microperfusion, physiological doses of peritubular or systemic angiotensin II stimulate proximal tubule transport (15-17). Systemic administration of the angiotensin II antagonist saralasin in whole animal studies decreased proximal tubule fractional and absolute volume reabsorption (22, 28).
Recently, the proximal tubule has been found to synthesize and
luminally secrete angiotensin II at concentrations ranging from 100- to
1,000-fold higher than that in plasma (4, 5, 27). This robust
endogenous production of angiotensin II within the proximal tubule is
consistent with an autocrine/paracrine role for endogenous angiotensin
II to regulate proximal tubule transport independent of systemic
angiotensin II. We recently demonstrated that blockade of the
production or action of endogenous angiotensin II in in vivo
microperfused proximal tubules by administration of luminal
108 M losartan or
104 M enalaprilat inhibited
the proximal tubule volume reabsorptive rate by 35-40% (23).
Our current data is consistent with an autocrine/paracrine role of angiotensin II in the regulation of proximal tubule transport by demonstration that the effect of luminal angiotensin II is regulated by acute changes in extracellular volume. The decrease in proximal tubule transport caused by luminal losartan is a measure of angiotensin II's contribution to regulation of proximal tubule transport. The proportionately greater decrease in transport observed with luminal losartan during volume contraction (58.0 ± 7.0 vs. 29.6 ± 9.0%, P < 0.05) indicates greater stimulation of net proximal tubule transport by luminal angiotensin II levels during acute volume contraction than during acute volume expansion.
The proposed autocrine or paracrine role for angiotensin II in the regulation of proximal tubule transport does not preclude the role of other systemic and peritubular physical factors that also concomitantly affect proximal tubule transport. Alterations in extracellular volume affect the systemic renin-angiotensin system, the permeability properties of the paracellular pathway, peritubular physical forces, renal nerve activity, and systemic catecholamine levels, which were not examined in this study (19). The net change in proximal tubule transport occurring with alterations in extracellular volume likely result from the combined effect of these systemic and peritubular factors, as well as endogenous proximal tubule angiotensin II.
Previous studies have demonstrated little or no effect of exogenous
luminal angiotensin II on proximal tubule transport in the hydropenic
rat (16, 23). To examine whether this was the result of elevated
endogenous production and luminal levels of angiotensin II during
volume contraction, we perfused angiotensin II into the lumen of
proximal tubules after acute volume expansion. The twofold increase in
volume reabsorption with addition of
108 M luminal angiotensin
II during volume expansion is consistent with endogenous physiological
concentrations of angiotensin II having a greater stimulatory effect on
volume absorption during volume contraction. Pharmacological or
subphysiological concentrations of exogenous luminal angiotensin II
(106 and
1010 M) had neither an
inhibitory nor stimulatory effect on proximal tubule volume
reabsorption.
The above data (Figs. 2 and 3) underscore the important and central role played by luminal angiotensin II levels. These data are supported by the results of two other recent studies that have examined the effect of changes in extracellular volume on luminal angiotensin II levels (4, 5). Braam et al. (5) found that, although not statistically significant, the luminal angiotensin II concentration in native tubular fluid fell from 14 nM during volume contraction to 8 nM after acute volume expansion. Conversely, Boer et al. (4) found that proximal tubule angiotensin II rose 3.5-fold when renal perfusion pressure was decreased 20%. This rise in angiotensin II with renal hypoperfusion and potential fall in angiotensin II with volume expansion are consistent with regulation of endogenously produced and luminally secreted angiotensin II by acute changes in extracellular volume. The absence of a statistically significant change in luminal angiotensin II levels induced by acute changes in extracellular volume in both studies might result from the lack of adequate sensitivity and precision in detecting small differences of luminal angiotensin II during different volume states. The small tubular fluid sample volumes along with sample dilution during the assay all contribute to variation in obtaining the final angiotensin II level. Such "background variation or noise" could potentially obscure any differences in luminal angiotensin II levels occurring between different volume states.
Alternatively, the decrease in luminal angiotensin II levels might represent dilution by the greater volume of tubular fluid rather than an actual decrease in production and secretion of angiotensin II. Regulation of the luminal concentration of angiotensin II may ultimately not be the modus operandi of endogenous proximal tubule angiotensin II. An alternate autocrine role for angiotensin II might involve regulation of transport by intracellular angiotensin II. Angiotensin II may be synthesized intracellularly and act within the proximal tubule cell to regulate transport independent of "extracellular" luminal angiotensin II levels. As an autocrine hormone, intracellular or tissue angiotensin II, rather than luminal angiotensin II, may fall with volume expansion and rise with volume contraction to regulate proximal tubule transport. In support of this notion, Boer et al. (4) also found that volume expansion markedly decreased the whole kidney tissue angiotensin II content, whereas reduced renal pefusion pressure raised whole kidney tissue angiotensin II.
Another equally plausible hypothesis to explain regulation of proximal
tubule transport by angiotensin II involves modulation of angiotensin
II receptor density or modulation of the sensitivity of the signal
transduction mechanism for angiotensin II. After changes in
extracellular volume, the effect of luminal angiotensin II would
"translate" into greater or lesser stimulation of proximal tubule
transport via alterations in receptor density or sensitivity of signal
transduction. Cheng et al. (8) recently found that angiotensin II
upregulates expression of angiotensin II receptors in the proximal
tubule. Thus the stimulation of proximal tubule transport by
angiotensin II could be significantly amplified via upregulation of its
own receptor. Our observations regarding heightened stimulation of
proximal tubule transport by endogenous angiotensin II during volume
contraction may, in part, result from an increase in angiotensin II
receptor expression caused by angiotensin II itself. Alternatively,
changes in extracellular volume might also alter the affinity of the
angiotensin II receptor for angiotensin II. Extracellular volume
expansion may decrease the angiotensin II receptor affinity, whereas
extracellular volume contraction may increase the angiotensin II
receptor affinity. This notion would reconcile the currently observed
stimulation of proximal tubule transport with
108 M angiotensin II in
volume-expanded but not volume-contracted rats with the previous
observation by Harris and Young (11) of stimulation of proximal tubule
transport with 109 M
angiotensin II in volume-contracted rats (11, 23). Although speculative, these possibilities provide an intriguing alternative to
the mechanism of action of endogenous angiotensin II.
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ACKNOWLEDGEMENTS |
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We are grateful for the able secretarial assistance of Patricia Wilson and Janell McQuinn and the technical assistance of Lisa K. Worrall.
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FOOTNOTES |
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This work was supported by a grant from the American Heart Association, Texas Affiliate (to A. Quan), National Institute of Diabetes and Digestive and Kidney Diseases Grant DK-41612 (to M. Baum), and by grants from the National Kidney Foundation of Texas (to A. Quan and M. Baum).
Address for reprint requests: A. Quan, Dept. of Pediatrics, UT Southwestern Medical Center, 5323 Harry Hines Blvd., Dallas, TX 75235-9063.
Received 22 July 1997; accepted in final form 6 March 1998.
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REFERENCES |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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 J. G. J. Hoenderop, B. Nilius, and R. J. M. Bindels Calcium Absorption Across Epithelia Physiol Rev, January 1, 2005; 85(1): 373 - 422. [Abstract] [Full Text] [PDF]
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A. Quan, S. Chakravarty, J.-K. Chen, J.-C. Chen, S. Loleh, N. Saini, R. C. Harris, J. Capdevila, and R. Quigley Androgens augment proximal tubule transport Am J Physiol Renal Physiol, September 1, 2004; 287(3): F452 - F459. [Abstract] [Full Text] [PDF]
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 R. Efendiev, C. E. Budu, A. R. Cinelli, A. M. Bertorello, and C. H. Pedemonte Intracellular Na+ Regulates Dopamine and Angiotensin II Receptors Availability at the Plasma Membrane and Their Cellular Responses in Renal Epithelia J. Biol. Chem., August 1, 2003; 278(31): 28719 - 28726. [Abstract] [Full Text] [PDF]
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D. Staahltoft, S. Nielsen, N. R. Janjua, S. Christensen, O. Skott, N. Marcussen, and T. E. N. Jonassen Losartan treatment normalizes renal sodium and water handling in rats with mild congestive heart failure Am J Physiol Renal Physiol, February 1, 2002; 282(2): F307 - F315. [Abstract] [Full Text] [PDF]
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A. Quan and M. Baum The renal nerve is required for regulation of proximal tubule transport by intraluminally produced ANG II Am J Physiol Renal Physiol, March 1, 2001; 280(3): F524 - F529. [Abstract] [Full Text] [PDF]
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E. Feraille and A. Doucet Sodium-Potassium-Adenosinetriphosphatase-Dependent Sodium Transport in the Kidney: Hormonal Control Physiol Rev, January 1, 2001; 81(1): 345 - 418. [Abstract] [Full Text] [PDF]
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A. Quan and M. Baum Renal nerve stimulation augments effect of intraluminal angiotensin II on proximal tubule transport Am J Physiol Renal Physiol, June 1, 2002; 282(6): F1043 - F1048. [Abstract] [Full Text] [PDF]
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P < 0.05, respectively). Magnitude of the decrement in volume reabsorption is
much greater during volume contraction than after volume expansion.
P < 0.05, compared with
volume-contracted control.
Jv)
observed with luminal perfusion of losartan in volume-contracted and
volume-expanded rats. Absolute decrease in volume reabsorption during
volume contraction (2.49 ± 0.46 nl · mm