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1 National Aeronautics and
Space Administration Ames Research Center, Following
spaceflight, changes in renal function of humans have been suggested.
To assess the effects of readaptation on renal function, urine was
collected from male rats (~245 g) over a 2-wk period following a
14-day spaceflight. Rats were assigned to three groups: flight animals
(n = 6), flight controls
(n = 6) housed in the flight cages on
the ground, and vivarium controls (n = 5) housed in standard shoe box cages. Animals were placed into individual metabolic cages for urine collection. Urine output was
significantly increased for 3 days following flight. Excretion rates of
Na+ and
K+ were increased, resulting in an
increased osmotic excretion rate. Creatinine excretion rate increased
over the first two postflight days. Glomerular filtration rate
increased immediately following spaceflight without changes in plasma
creatinine, Na+,
K+, or osmolality. Increased
excretion of solute was thus the result of increased delivery and a
decreased percent reabsorption of the filtered load. Osmolal clearance
was increased immediately postflight while free water clearance was
decreased. In growing rats, the diuresis after short-duration
spaceflight is the result of an increase in solute excretion with an
accompanying reduction in free water clearance.
urinary sodium and potassium excretion; aldosterone; free water
clearance; osmolal clearance
RENAL FUNCTION HAS BEEN reported to be altered
following return to Earth from spaceflight (6, 12, 14, 18, 22). In
humans, urine flow rate is decreased or not changed, and concentrating ability is reduced (8-10, 12-14, 18-20). These changes
are postulated to be related to a decrease in sensitivity to
vasopressin and a decrease in the concentration gradient in the renal
medulla. Reports of rats following spaceflight suggest that urine flow rate is not changed, but the renal handling of solutes is altered (6,
7, 18, 19). Postflight, there is an increase in the percent of filtered
sodium and potassium loads excreted; animals in one of these studies,
however, had a period of limited access to water and were not evaluated
over the first 48 h after flight (6, 7, 19).
Assessment of renal function in humans during spaceflight has been
compromised by a variety of factors, including motion sickness, subject
compliance, and the use of countermeasures such as exercise (9, 13,
15). At the onset of spaceflight, there is a cephalic shift of fluids
in humans (31). This redistribution is purported to induce a diuresis;
in-flight measurements, however, have not demonstrated an increase in
urine output (8, 10, 12, 14). Furthermore, the decrease in total body
water appears to be the result of a reduction in intake (14, 31). In
response to a saline infusion during spaceflight, excretion of the
fluid load was delayed and attenuated (21). These changes would affect the ability to regulate fluid and electrolyte homeostasis in response to redistribution of body fluids on return to Earth.
The rat hindlimb suspension model has been used to study many of the
changes associated with spaceflight, including fluid and electrolyte
homeostasis (3, 4, 28, 32). Tucker and Mendonca (26, 27) have evaluated
the effects of this model on renal function, assessing the effects of
reloading (simulating return to Earth) on animals after 14 and 30 days
of suspension. Over the first 24 h of reloading, no change in the urine
flow rate occurs despite an increase in glomerular filtration rate.
The present study was undertaken to
1) evaluate renal responses in rats
following spaceflight and 2)
identify specifically the changes in handling of solutes and the
contributions of solutes to observed changes in urine flow rate. We
hypothesized that, following spaceflight, there would be an
antidiuresis in the rats primarily due to reduction in osmolal
clearance. Animals were evaluated for 14 days following a 14-day
spaceflight.
Studies were conducted on specific pathogen-free Sprague-Dawley-derived
rats (Harlan Laboratories, Prattsville, AL) received 8 days before
launch when the animals were 30 days of age and weighed ~100 g. All
animal protocols were approved by the appropriate National Aeronautics
and Space Administration (NASA) Animal Care Committees and adhere to
the National Institutes of Health guidelines for the humane care and
use of animals.
Experimental procedures. Animals were
arranged by descending weight and randomly assigned to three groups so
that each group had the same initial mean body weight. The groups were
flight, flight control, and vivarium control. Flight animals were
individually housed and flown in a Research Animal Holding Facility,
and flight control animals were individually housed in
flight-simulation cages (~4 in. high by 4 in. wide by 12 in. deep;
the height of these cages does not allow the animals to rear on their
hind legs). All animals were maintained on the same 12:12-h light-dark
cycle to which they were entrained before selection for the study. Both groups were fed food bars [Teklad (Madison, WI) NASA Experimental Rodent Diet no. TD 88179 extruded into food bars, dipped in 15% sorbate to retard mold growth, radiation sterilized, sealed in polyethylene bags, and stored at 4°C until use] and provided
water ad libitum. Vivarium control animals were individually housed two
animals per cage in standard shoe box cages (8 in. high by 10.5 in.
wide by 19 in. deep) with a Plexiglas divider running parallel to the
long axis of the cage to separate the two rats; vivarium controls were
fed pieces of flight food bars (Teklad) and provided water ad libitum.
Flight animals were flown aboard the Space Shuttle Columbia (STS-58)
for 14 days. Initially there were 12 animals per group. On landing of
the shuttle (R + 0), the animals underwent an examination by a
veterinarian to assess their health and were turned over to the
investigator within 6 h of landing. One-half of the animals from each
group were then anesthetized with Metofane, and blood samples were
taken. The remaining six animals in each group were placed in metabolic
cages for the next 14 days. One vivarium control rat was removed from the study because it failed to gain weight when transitioned to the
metabolic cage. Animals were provided a powdered diet (Teklad diet no.
TD 88179) and water ad libitum. The animals were maintained on a
12:12-h light-dark cycle [lights on at 5:00 AM, lights off at
5:00 PM, Pacific Standard Time (PST)]. For the first week, the
body weight of each animal was measured daily using an electronic balance; during the second week, the rats were weighed twice
(day 9 and
day
14). Food consumption and water
consumption were determined by weighing the food and water containers
on an electronic balance. Urine volumes were measured with a graduated
cylinder. Over the first 4 days postflight, urine collections were
taken twice a day at 5:30 AM (AM) and 3:30 PM (PM), PST. The AM
collection covered the active period for rats. On all subsequent days,
collections occurred at 3:30 PM. Daily collections were taken on
days
5-7. Pooled 2-day collections were obtained on
days
9,
11, and
13. A final 24-h collection was made
on day
14. Data in the text are corrected for
collection duration. On day
14, the animals were anesthetized by
inhalation of Metofane until sedated, and blood samples were taken.
Sample handling. Blood was taken from
the descending aorta of anesthetized animals at recovery (R + 0) and 14 days after landing (R + 14), six animals per group per time period.
Blood was placed in serum separator tubes, refrigerated, and allowed to
clot for 2 h. Samples were then centrifuged in a refrigerated (4°C)
centrifuge, and aliquots of serum were frozen at Calculations and statistics. Urine
flow rate (V) was calculated as the volume collected divided by the
time duration of the collection. The rate of excretion of a substance
was the urine concentration times V. Because blood samples were not
obtained on the animals in the metabolic cages, the mean serum
concentration obtained from animals during postflight procedures were
used to calculate clearance rates. Osmolal clearance
(Cosm) was calculated as the
rate of osmotic excretion divided by the mean serum osmolality. Free
water clearance was equal to V A two-way ANOVA was used to compare the blood samples between groups,
and immediately postflight versus after 14 days of recovery. A two-way
ANOVA adjusted for repeated measures over time was used in the analysis
of the urine data. Differences between means were determined by the
Tukey-Kramer test on individual data. A probability of <0.05 was
accepted as being significant. Values in the text are means ± SE.
Serum osmolality and serum concentrations of creatinine, sodium,
potassium, and calcium were not significantly different among the
groups of animals (Table 1), nor were there
differences in osmolality and concentrations of sodium, potassium, or
calcium determined immediately postflight compared with those
determined after 14 days of recovery. Serum creatinine levels for
flight animals, although not different among groups on R + 0, were
elevated compared with those obtained for flight animals
following recovery on R + 14.
ABSTRACT
Top
Abstract
Introduction
Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Methods
Results
Discussion
References
METHODS
Top
Abstract
Introduction
Methods
Results
Discussion
References
20°C for
later analysis. Urine was collected at room temperature in vials
containing 50 µl of Traysol (aprotinin; Bayer, West Haven, CT);
Traysol was added at the request of other investigators who shared the
samples. Aliquots of the daily urine sample were taken and frozen at
20°C. Serum and urine concentrations of creatinine, sodium,
potassium, and calcium were measured using an automated analytical
system (COBAS; Roche Diagnostic Systems, Somerville, NJ). Serum and
urine osmolalities were measured by freezing-point depression (Advanced Instruments, Needham Heights, MA). Urine aldosterone concentration was
measured by radioimmunoassay (Diagnostic Products, Los Angeles, CA)
following extraction.
Cosm. Glomerular filtration rate
(GFR) was estimated from the clearance rate of creatinine (creatinine
excretion rate divided by serum concentration). The percent of the
filtered load excreted for a substance was calculated as the rate of
excretion × 100 divided by the serum concentration × GFR.
RESULTS
Top
Abstract
Introduction
Methods
Results
Discussion
References
Table 1.
Serum levels at two time points
Body weight was not different among groups before flight (flight animals: 137 ± 1.8 g; flight controls: 137 ± 2.1 g; vivarium controls: 136 ± 2.9) and immediately on recovery (Table 2). Weight gain (the daily change in body weight) decreased in flight animals within 24 h after landing compared with both control groups (Table 2; Ref. 29). Water intake did not differ between groups or over time (Table 2). The decrease in weight gain in flight animals was associated with a significant reduction in food consumption over the first 2 days of recovery compared with both control groups (Table 2). The decrease in mean food consumption of the flight group compared with control groups during this 48-h period, ~10 g, could not solely account for the 20-g difference in body weight gain of flight animals compared with flight controls or 31 g compared with vivarium controls. The other factor contributing to the reduction in body weight of flight animals was an increase in urine volume of 31 ml over the first 48 h of recovery compared with the mean excretion rate for flight control animals. The increase in V of flight animals persisted for at least 3 days postspaceflight (Fig. 1, Table 2).
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The daily creatinine excretion rate of flight animals was increased postflight for 2 days (Fig. 1). In the flight animals, osmotic excretion was increased above both flight and vivarium controls for 3 days postflight (Fig. 2). The daily rate of sodium excretion of flight animals was significantly increased only on day 1 of recovery, whereas potassium excretion of flight animals was elevated for 2 days (Fig. 2). The only significant group effect was for daily potassium excretion, with flight animals having a greater excretion rate compared with both groups of controls. Calcium excretion showed an effect of caging during the flight period, as both the flight and flight control animals had reduced initial values compared with vivarium controls (Fig. 2). Flight animals were thus compared directly with flight control animals. There was an increase in daily calcium excretion in both flight and flight control animals compared with vivarium control animals over the subsequent 2 days, with flight animals increasing more than flight controls on day 5. The calcium excretion rates of flight animals returned to levels comparable to vivarium controls, whereas flight control values remained elevated for the next 3 days. An increase in the excretion rate of aldosterone in flight animals was noted for 2 days postflight (Fig. 3).
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Clearance rates were calculated for the first 24 h using the mean serum concentration [no difference was noted in serum concentrations immediately postflight among groups (Table 1)] and in the urine excretion rate for a group (Fig. 2). Cosm was increased in the flight animals compared with both control groups (Fig. 4). Free water clearance was more negative in the flight animals compared with the control groups.
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The differences in excretion in flight animals may be due to increases in GFR (Fig. 5) as indicated by the increase in the creatinine excretion rate (Fig. 1). The clearance of creatinine was assumed to be indicative of GFR. The ratio of urinary concentration of solutes to creatinine concentration was compared to correct for possible differences in filtration rates thus reflecting renal handling of the solute as serum levels were not changed. On day 1, the urinary sodium-to-creatinine ratio was increased for flight animals (0.9 ± 0.06) compared with the ratios for flight and vivarium controls (0.4 ± 0.17 and 0.4 ± 0.12, respectively), indicative of an increase in the percent of the fluid load excreted. Differences were not observed in the ratios of potassium, calcium, or osmolality to creatinine.
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During recovery, diurnal variations in renal function in all groups were noted (Table 3). There were increases in excretion rates during the period from 3:30 PM to 5:30 AM (AM), which included the time when the lights were off. In the flight animals, V was increased for 3 days postflight during the AM period compared with both control groups. V in flight animals was increased during the PM period only on days 1 and 2. There were increases in creatinine, potassium, and osmotic excretion rates of flight animals during the AM period, with smaller increases noted over the PM period. However, the magnitude of the diurnal changes for flight animals compared with flight control values was similar for AM and PM. Calcium excretion showed no diurnal effect. The increase in sodium excretion on day 1 was predominately due to a fivefold increase in excretion during the PM period, but a twofold increase was also noted in the AM.
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DISCUSSION |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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In the conduct of research on the effects of spaceflight, there are severe constraints: a limited number of specimens are available and access to the specimens during flight is restricted. At present, there is no method for collecting urine samples from rats during spaceflight that would allow the study of renal function during flight. In addition, numerous investigators are usually studying the same specimen, which, although permitting integration of data among studies, may cause one study to impact another. In the present study, the animals and samples were shared with other investigators. The amount of urine and blood samples available to us was limited. Access to future spaceflights to confirm the present findings is years off. The present study, although not optimal, allowed the effects of reloading on return to Earth on renal function of rats to be evaluated.
The data from this experiment strongly suggest that changes in renal function of growing rats occur immediately after spaceflight. Urine flow, creatinine clearance (i.e., GFR), Cosm, sodium excretion, potassium excretion, and aldosterone excretion increase in the first 24 h postflight.
Following spaceflight, rats exhibited an increase in V that persisted for over 48 h. This increase coupled with a reduction in food intake resulted in a decrease in body weight. The increase in V appears to be the result of an increase in the clearance of osmotic substances, specifically sodium in the first 24 h and potassium over the first 48 h. When corrected for creatinine clearance, only sodium remained elevated, suggesting that the other solutes showed differences due to changes in the rate of filtration rather than renal tubular handling.
Earlier studies of postspaceflight rats showed no difference in V, but the data were not collected until 40 h after spaceflight (6, 7, 18). However, a decrease in the ability to handle a water load was noted (6, 7, 18). In humans, a decrease in V following spaceflight was reported; however, these individuals had an increase in plasma osmolality indicative of dehydration (18, 20). In the present study, no differences were noted in serum osmolality, yet V in flight animals was increased approximately twofold for 2 days following spaceflight compared with both control groups. The increase in V was in contrast to hypothesized changes. In spaceflight, blood volume and total body water have been reported to be reduced in humans (24, 29). On return to the gravity of Earth, fluids move from the core of the body to the extremities (31). This shift, coupled with the reduction of body water during flight, would be expected to initiate the conservation of fluids by the kidneys. In rats, this does not appear to occur and may be the result of changes in the sensitivity of volume receptors or the sequestration of fluids in the periphery (31). Furthermore, in quadrupeds such as the rat, fluid loss may not occur in spaceflight.
An increase in GFR may contribute to an increase in V. The clearance of creatinine is often used as an indicator of GFR. In the present study, the increase in the excretion of creatinine may be indicative of an increase in GFR, as serum concentrations are not significantly different postflight between groups. However, plasma creatinine concentrations of rats are reported to be increased when measurements are obtained 11-40 h postlanding (11, 16). Furthermore, there are indexes of muscle damage immediately postflight that would contribute to an increase in plasma and urine creatinine concentrations (25). In the present study, serum creatinine concentrations were increased in flight animals immediately postflight compared with levels obtained after 14 days of recovery (Table 1). There are limitations to interpretation of the present data because plasma samples for determination of creatinine concentrations came from one group of animals and urine levels were measured in another. Although our data are characteristic of an increase in GFR, which could contribute to the increase in V, this increase in filtration has to be confirmed by direct measurement.
The increase in V in the first 24 h is due to an increase in Cosm. This increase in Cosm appears to be the result of a natriuresis with a secondary kaluresis. The increase in the excretion of sodium appears to be rectified within 24 h, possibly due to the increase in aldosterone as indicated by an increase in its excretion in urine. The conservation of sodium by the actions of aldosterone may contribute to the excretion of potassium. Flight animals had a greater total excretion of potassium over the 14-day recovery period compared with both control groups. However, this may also be the product of muscle damage (25). Of note is that the increase in the excretion of both creatinine and potassium occurred in the AM, lights-off period, which would have been the active weight-bearing period for the rats. The increase in the excretion of potassium may also result from a change in the concentrating mechanisms in the kidney. Gazenko et al. (6, 7) found a decrease in the ability of flight rats to handle a potassium load and postulated that this was the result of the observed decrease of potassium concentration in the outer zone of the renal medulla (23). These investigators also noted a postflight difference in the handling of sodium following a water load. Sodium retention was decreased in the flight animals. The reason for the increase in solute excretion following spaceflight in the present study is not clear, but solute excretion appears to be the primary component of the increase in V.
The increased excretion of sodium in the presence of an elevated excretion of aldosterone may appear paradoxical. In response to an increased sodium loss via the kidneys following landing, circulating aldosterone concentrations would be increased and a concomitant increase in urinary aldosterone levels would be observed. However, the actions of increased aldosterone concentration may have been delayed for hours because of the latency time necessary for protein synthetic responses to be initiated (17). Furthermore, the increase in aldosterone persisting for 2 days suggests a possible role in the correction of the renal handling of sodium, but the actions of aldosterone may have been delayed initially.
Natochin et al. (18-20) have reported decreased renal concentrating ability in both rats and humans postspaceflight. In rats, they found a disruption of tubular reabsorption of water; specifically, the ability to produce a concentrated urine was altered due to a decrease in the sensitivity of the kidney to vasopressin (antidiuretic hormone). In contrast, we found free water clearance to be decreased postflight. That is, there was an increase in the tubular reabsorption of water. This suggests that the flight rats still had the ability to form a concentrated urine and the differences in V were predominantly due to a decreased reabsorption (increased excretion) of osmotically active substances.
In both flight and flight control animals, the excretion of calcium was reduced compared with that of vivarium controls, suggesting an effect of the limited cage space. Recent studies show that there is a difference in response of the muscles of animals flown in space depending on how they are housed (25). For these reasons, we compared the calcium excretion rates of the flight animals only with the calcium excretion rates of flight controls. In both of these groups, there was a time effect. Following the transfer into the larger metabolic cages, both groups increased the excretion of calcium for 3 days. After this period, the flight animals dramatically reduced their calcium excretion while the flight control animals had a slow decrease. There was a group effect noted, with the flight animals having a reduced calcium excretion over the 14 days of recovery compared with the flight controls. The renal conservation of calcium postflight would agree with an increase in the remodeling of bone during this period (2).
Over the first 4 postflight days, urine samples were taken twice a day. In all groups, a distinct diurnal pattern in urine excretion rate is observed: an increase in urine flow during the AM lights-off collection period compared with the PM lights-on collection period. Rats are nocturnal animals, and the AM collection period includes their active period. Although recovery from spaceflight appeared to disrupt renal function, it did not affect the diurnal cycle. Others have shown changes in the diurnal temperature cycles of animals resulting from spaceflight, but the change in diurnal cycle does not appear to be reflected in renal function changes (4). However, renal function cycles are less sensitive than temperature cycles to diurnal changes.
Our findings of alterations of renal function postflight are in contrast to those previously reported. These differences may be due to the earlier access to our animals (within 3 h) compared with the delays in access to animals in previous studies. Our animals also had continuous availability of food and water. In other studies, animals have had periods of no access to food and water, a condition that, while also mimicked in the control groups, could have produced a different response in subsequent evaluations.
In summary, on return of rats to Earth following 14 days of spaceflight, there are significant alterations in renal function. The initial diuresis appears to be due to an increased osmolal clearance coupled to a natriuresis and kaluresis. The natriuresis is attenuated within 24 h, probably due to increased aldosterone. There is an increase in water reabsorption, compensating in part for obligatory losses associated with the reduction in solute reabsorption. However, there is still a net increase in the renal loss of fluids and electrolytes, contributing to a decrease in body weight (30). The alteration in the renal handling of fluid and electrolytes, resulting in a net loss of fluids in rats on return to Earth, is in conflict with existing theories of fluid shifts during spaceflight (31). It is possible that rats do not lose fluids during flight and may, in fact, retain fluids. In a recent experiment, the body weight of rats appeared to be increased when measured during exposure to spaceflight (1). This increase in body weight could be related to an increase in total body water. Our observations suggest possible changes in other homeostatic mechanisms of rats during and after spaceflight that need further investigation if this animal continues to be a primary model for study.
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FOOTNOTES |
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Address for reprint requests: C. Wade, NASA Ames Research Center, Life Sciences Division MS-239-11, Moffett Field, CA 94035-1000.
Received 21 May 1997; accepted in final form 24 June 1998.
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REFERENCES |
|---|
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Top
Abstract
Introduction
Methods
Results
Discussion
References
|
|---|
1.
Allebban, Z.,
L. A. Gibson,
R. D. Lange,
T. L. Jago,
K. M. Strickland,
D. L. Johnson,
and
A. T. Ichiki.
Effects of spaceflight on rat erythroid parameters.
J. Appl. Physiol.
81:
117-122,
1996
2.
Bikle, D. D.,
J. Harris,
B. P. Halloran,
and
E. Morey-Holton.
Altered skeletal pattern of gene expression in response to spaceflight and hindlimb elevation.
Am. J. Physiol.
267 (Endocrinol. Metab. 30):
E822-E827,
1994
3.
Deavers, D. R.,
X. J. Musacchia,
and
G. A. Meininger.
Model for antiorthostatic hypokinesia: head-down tilt effects on water and salt excretion.
J. Appl. Physiol.
49:
576-582,
1980
4.
Fuller, C. A.,
D. M. Murakami,
and
F. M. Sulzman.
Gravitational biology and the mammalian circadian timing system.
Adv. Space Res.
9:
283-292,
1989.[Medline]
5.
Gauquelin, G.,
E. L. Schiffrin,
R. Garcia,
M. Entresangles,
M. Cantin,
and
C. Gharib.
Specific bonding of natriuretic factor to renal glomeruli during day or night antiorthostatic suspension in the rat.
Life Sci.
43:
1905-1912,
1988[Medline].
6.
Gazenko, O. G.,
A. Grigoriev,
and
Y. V. Natochin.
Fluid-electrolyte balance and spaceflight.
In: Problems in Space Biology. Moscow: Nauka, 1986, vol. 54, p. 1-238.
7.
Gazenko, O. G.,
Y. V. Natochin,
Y. A. Ilyin,
N. A. Ilyushko,
Y. I. Kondratiev,
Y. A. Lavrova,
and
Y. I. Shakhmatova.
Fluid-electrolyte metabolism and renal function of white rats in experiments aboard Cosmos biosatellites.
Aviat. Space Environ. Med.
55:
685-691,
1984[Medline].
8.
Gazenko, O. G.,
E. B. Schulzhenko,
A. I. Grigoriev,
O. Y. Atkov,
and
A. D. Egorov.
Review of basic medical results of the Salyut-7-Soyuz-T 8-month manned flight.
Acta Astronaut.
17:
155-160,
1988.[Medline]
9.
Grigoriev, A. I.
Correction of changes in fluid-electrolyte metabolism in manned space flights.
Aviat. Space Environ. Med.
54:
318-323,
1983[Medline].
10.
Grigoriev, A. I.,
I. A. Popova,
and
A. S. Ushakov.
Metabolic and hormonal status of crewmembers in short-term spaceflights.
Aviat. Space Environ. Med.
58:
A121-A125,
1987[Medline].
11.
Grindeland, R. E.,
I. A. Popova,
M. Vasques,
and
S. B. Arnaud.
Cosmos 1887 mission overview: effects of microgravity on rat body and adrenal weights and plasma constituents.
FASEB J.
4:
105-109,
1990[Abstract].
12.
Leach, C. S.
Medical results from STS 1-4: analysis of body fluids.
Aviat. Space Environ. Med.
54:
S50-S54,
1983[Medline].
13.
Leach, C. S.
Fluid control mechanisms in weightlessness.
Aviat. Space Environ. Med.
58:
A74-A79,
1987[Medline].
14.
Leach, C. S.,
and
P. C. Rambout.
Biomedical responses of the Skylab crewman: an overview.
In: Biomedical Results From Skylab, edited by R. S. Johnston,
and L. F. Dietlein. Washington, DC: National Aeronautics and Space Administration, 1977, p. 204-216.
15.
Maillet, A.,
G. Gauquelin,
D. Vorobiev,
J. O. Fortrat,
R. L. Hughson,
J. Frutoso,
A. M. Allevard,
R. Cartier,
M. Patricot,
A. Koulev,
R. Kvetnansky,
A. Kotovskaya,
A. I. Grigoriev,
and
C. Gharib.
Blood volume regulating hormones, fluid and electrolyte modifications, heart rate variability during 14-day and 176-day space flights (Antares-Mir-92).
In: Proc. Eur. Symp. Life Sci. Res. Space 5th Arcachon, France, 1994, p. 261-267.
16.
Merrill, A. H., Jr., E. Wang, R. E. Mullins,
R. E. Grindeland, and I. A. Popova. Analyses
of plasma for metabolic and hormonal changes in rats flown aboard
COSMOS 2044. J. Appl. Physiol. 73, Suppl.: 132S-135S, 1992.
17.
Morris, D. J.
The metabolism and mechanisms of action of aldosterone.
Endocr. Rev.
2:
234-247,
1981[Medline].
18.
Natochin, Y. V.,
A. Grigoriev,
V. B. Noskov,
R. G. Parnova,
Y. V. Sukhanov,
D. L. Firsov,
and
E. I. Shakhomatova.
Mechanism of postflight decline in osmotic concentration of urine in cosmonauts.
Aviat. Space Environ. Med.
62:
1037-1043,
1991[Medline].
19.
Natochin, Y. V.,
A. I. Grigoriev,
and
L. V. Serova.
The influence of space flight on water-salt homeostasis in man and animals.
In: Proc. Eur. Symp. Life Sci. Res. Space 3rd Graz, Austria, 1987, p. 259-261.
20.
Natochin, Y. V.,
G. I. Kozyrevskaya,
and
A. I. Grigoryev.
Study of water-salt metabolism and renal function in cosmonauts.
Acta Astronaut.
2:
175-188,
1975.[Medline]
21.
Norsk, P.,
C. Drummer,
L. Rocker,
F. Strollo,
N. J. Christensen,
J. Warberg,
P. Bie,
C. Stadeager,
L. B. Johansen,
M. Heer,
H.-C. Gunga,
and
R. Gerzer.
Renal and endocrine responses in humans to isotonic saline infusion during microgravity.
J. Appl. Physiol.
78:
2253-2259,
1995
22.
Norsk, P.,
and
M. Epstein.
Manned space flight and the kidney.
Am. J. Nephrol.
11:
81-97,
1991[Medline].
23.
Pankova, A. S.
Morphological study of rat kidneys after flight aboard the Cosmos-936 biosatellite.
Kosmicheskaya Biologiya I Aviakosmicheskaya Meditsina
14:
26-31,
1980.
24.
Pitts, G. C.,
A. S. Ushakov,
N. Pace,
A. H. Smith,
D. F. Rahlmann,
and
T. A. Smirnova.
Effects of weightlessness on body composition in the rat.
Am. J. Physiol.
244 (Regulatory Integrative Comp. Physiol. 13):
R332-R337,
1983
25.
Riley, D. A.,
S. Ellis,
G. R. Slocum,
F. R. Sedlak,
J. L. W. Bain,
B. B. Krippendorf,
C. T. Lehman,
M. Y. Macias,
J. L. Thompson,
K. Vijayan,
and
J. A. De Bruin.
In-flight and postflight changes in skeletal muscles of SLS-1 and SLS-2 spaceflown rats.
J. Appl. Physiol.
81:
133-144,
1996
26.
Tucker, B. J.,
and
M. M. Mendonca.
Alterations in glomerular and tubular dynamics at 1 and 14 days simulated microgravity and after acute return to orthostasis.
J. Gravitational Physiol.
2:
P31-P32,
1995.[Medline]
27.
Tucker, B. J.,
and
M. M. Mendonca.
Effects of 30 day simulated microgravity and recovery on fluid homeostasis and renal function in the rat.
J. Gravitational Physiol.
2:
P33-P34,
1995.[Medline]
28.
Tucker, B. J.,
C. A. Mundy,
M. G. Ziegler,
C. Baylis,
and
R. C. Blantz.
Head-down tilt and restraint on renal junction and glomerular dynamics in the rat.
J. Appl. Physiol.
63:
505-513,
1987
29.
Udden, M. M.,
T. B. Driscoll,
L. A. Gibson,
C. S. Patton,
M. H. Pickett,
J. B. Jones,
R. Nachtman,
Z. Allebban,
A. T. Ichiki,
R. D. Lange,
Blood volume and erythropoiesis in the rat during spaceflight.
Aviat. Space Environ. Med.
66:
557-561,
1995[Medline].
30.
Wade, C. E., J. S. Harper, N. G. Dauton, M. L. Corcoran, and E. Morey-Holton. Body mass
gain during altered gravity: spaceflight, centrifugation, and return to
1 G. J. Gravitational Physiol. In
press.
31.
Watenpaugh, D. E.,
and
A. R. Hargens.
The cardiovascular system in microgravity.
In: Handbook of Physiology. Environmental Physiology. Bethesda, MD: Am. Physiol. Soc., 1996, sect. 4, vol. I, chapt. 29, p. 631-674.
32.
Wronski, T. J.,
and
E. R. Morey-Holton.
Skeletal response to simulated weightlessness: a comparison of suspension techniques.
Aviat. Space Environ. Med.
58:
63-68,
1987[Medline].
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