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First published online June 27, 2008
Journal of Experimental Biology 211, 2327-2335 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.016832
Effects of salinity on intestinal bicarbonate secretion and compensatory regulation of acid–base balance in Opsanus beta
University of Miami, Rosenstiel School of Marine & Atmospheric Science, 4600 Rickenbacker Causeway, Miami, FL 33419-1098, USA
* Author for correspondence (e-mail: jgenz{at}rsmas.miami.edu)
Accepted 12 May 2008
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Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Key words: osmoregulation, HCO3– secretion, toadfish, fractional water absorption, drinking rate
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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300–350 mosmol l–1, approximately one-third
that of seawater (1000 mosmol l–1)
(Shehadeh and Gordon, 1969
).
This results in a constant diffusive salt gain from the surrounding
environment, as well as osmotic water loss, for which fish compensate by
drinking seawater. Water absorption is driven by active uptake of ions by the
gastrointestinal tract (Smith,
1930), particularly Na+ and Cl–
absorption across the intestinal epithelium
(Skadhauge, 1974;
Ando et al., 1975). A large
portion of intestinal Cl– absorption results from apical
Cl–/HCO3– exchange
(Ando and Subramanyam, 1990;
Wilson et al., 1996;
Grosell et al., 2001;
Grosell et al., 2005), which
occurs in excess and independently of Na+ absorption (reviewed by
Grosell, 2006). The secreted
HCO3– has two sources: hydration of endogenous
metabolic CO2 (Wilson and
Grosell, 2003; Grosell et al.,
2005; Grosell and Genz,
2006), mediated by carbonic anhydrase
(Grosell et al., 2005), and
extracellular HCO3– transport across the
basolateral membrane, presumably by
Na+/HCO3– cotransport
(Ando and Subramanyam, 1990;
Grosell and Genz, 2006). The
contribution of HCO3– derived from each of these
two sources varies among species (Grosell,
2006), but each source accounts for approximately 50% of
intestinal HCO3– secretion in the gulf toadfish,
Opsanus beta (Grosell and Genz,
2006). In O. beta, the H+ liberated by
intracellular carbonic anhydrase-mediated CO2 hydration is
transported across the basolateral membrane into the extracellular fluids
(Grosell et al., 2001) in
exchange for Na+ (Grosell and
Genz, 2006) and results in net acid absorption
(Grosell and Taylor, 2007)
proportional to the HCO3– secretion driving
intestinal fluid absorption.
Fish maintain relatively alkaline blood pH, ranging in most cases from 7.7
to 8.1 depending on temperature, primarily by transfer of acid–base
molecules across the gill epithelium by mitochondrion-rich cells
(Marshall and Grosell, 2005;
Evans et al., 2005). Due to
high solubility in water, the unidirectional movement of water across the
respiratory surface and the countercurrent blood and water flow at the gill,
molecular CO2 from the blood is readily excreted into the water
during gas exchange with carbonic anhydrase-rich erythrocytes, resulting in
low plasma CO2 partial pressure
(PCO2) compared with air-breathing vertebrates
(Heisler, 1980;
Claiborne, 1997).
Hyperventilation to combat acidosis is therefore a relatively inefficient
strategy in water-breathing compared with air-breathing animals due to the
lower scope for change in PCO2. Instead, the
main response to a metabolic acidosis in teleost fish is increased acid
excretion across the gill epithelium
(McDonald et al., 1982;
Evans, 1982;
Claiborne, 1997). Both
Na+/H+ exchange and V-type H+-ATPase excrete
H+ from the gill, while the primary mechanism for base excretion at
the gill is apical Cl–/HCO3–
exchange (Claiborne et al.,
1997; Claiborne et al.,
2002).
Changes in intestinal base secretion rates associated with osmoregulatory
processes would be expected to have an impact on whole-animal acid–base
balance. Higher drinking rate in elevated salinity is predicted, due to
greater diffusive fluid loss, and fish exposed to high salinity are also
predicted to increase HCO3– secretion into the
intestinal lumen to facilitate water absorption
(McDonald and Grosell, 2006;
Grosell, 2006). Increased
intestinal HCO3– secretion creates a potential
problem, as it results in systemic acid gain and the possibility of metabolic
acidosis. A compensatory mechanism may exist to avoid disturbance of systemic
acid–base balance caused by changes in intestinal base secretion, and,
if present, this mechanism would likely occur at the gill, the primary
acid–base regulatory tissue in fish.
To investigate the impact of high or low salinity on
HCO3– secretion into the intestinal lumen, and
subsequent systemic acid–base consequences, we collected the rectal
fluids excreted by gulf toadfish acclimated to 9, 35 and 50 ppt. The
extracellular fluids of the fish are isosmotic to the surrounding water at 9
ppt, reducing the need to drink. Conditions naturally experienced by the gulf
toadfish are represented by 35 ppt, while 50 ppt represents a high salinity
tolerance limit, intended to osmotically stress the fish and increase
intestinal HCO3– secretion above usual rates
(McDonald and Grosell, 2006)
without causing severe disturbance of salt and water balance. As predicted,
ambient salinity was observed to strongly influence rectal base excretion, and
the hypothesis of extra-intestinal compensation was therefore examined by
measurements of net, extra-intestinal acid fluxes at 9, 35 and 50 ppt.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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). Toadfish were held in tanks that had continuous flow of
aerated, filtered seawater from Biscayne Bay (Bear Cut, 34–37 ppt,
22–26°C) for at least two weeks before experimentation. Segments of
polyvinyl chloride tubing were provided for shelter and the fish were fed
pieces of squid until satiation twice weekly, but were starved for 48 h prior
to sampling. Fish were maintained in the lab and used according to an approved
University of Miami animal care protocol (IACUC #05-251).
Determination of drinking rate
The method used to determine drinking rate in toadfish acclimated to 50 ppt
(N=8) was adapted from a previously published method
(Grosell et al., 2004). Fish
were allowed to acclimate overnight to a smaller (5 l) glass container to
facilitate efficient isotope use, after which water flow was stopped and
3.7x105 Bql–1 [14C]polyethylene
glycol-4000 (PEG-4000) (specific activity: 7.585 Bq g–1;
NEN-Dupont, Boston, MA, USA) was added to the tank. Following a 6.1 h
exposure, during which water samples were taken at 0.25 and 6.1 h, tricaine
methane sulfonate (MS-222) was added to the tank to a final concentration of
0.2 g l–1, euthanizing the fish, which were removed
individually from the tank, rinsed with non-radioactive 50 ppt seawater,
weighed (22.3±1.3 g) and sampled. Sampling consisted of clamping the
gastrointestinal tract at the start of the esophagus and immediately anterior
to the anus by hemostats to prevent loss of fluid, and removal of the entire
gastrointestinal tract from the body. Gastrointestinal samples were weighed,
homogenized and digested in 10 ml H3PO4 (3% v/v) and
prepared for analysis by combining 1 ml aliquots of supernatant from each
homogenized sample with 4 ml of 50 ppt seawater. A 14C-free 5 ml 50
ppt sample served as blanks for these analyses. A 1 ml aliquot of each water
sample was diluted to 5 ml total volume with 50 ppt seawater; β
radioactivity was determined for all samples by liquid scintillation counting
using a TmAnalytic BetaTract 6895 instrument (Elk Grove Village, IL, USA). No
quenching was observed. Drinking rate (ml kg–1
h–1) was calculated from the radioactivity in digested
gastrointestinal tissue samples and that of water samples, mass of individual
fish, including the mass of the gastrointestinal tissue, and exposure time.
The total activity of the GI tract was determined from the total volume of
tissue homogenate (mass of tissue and fluid + H3PO4) and
the activity recorded in the 1 ml aliquot. Note that this procedure has been
verified with respect to absence of [14C]PEG in plasma and rectal
fluids at the end of the 6 h incubation period for toadfish exhibiting
drinking rates as high as in the present study
(Grosell et al., 2004).
Acute transfer to hypersalinity
Toadfish were kept in a 103-liter aquarium with filtered seawater (35
ppt) on a flow-through system, as described above. Water flow was terminated
and approximately 80% of the water was siphoned off and replaced with a
mixture of sea salt (Instant Ocean®; Aquarium Systems Inc., Mentor, OH,
USA) dissolved in 35 ppt seawater to give a final salinity of 60 ppt. Fish
were acutely transferred to 60 ppt, as it was observed that this procedure
could be tolerated by non-cannulated fish. Fish (N=8) were sampled
immediately before transfer to 60 ppt and at 6, 24 and 96 h post-transfer.
Blood samples (200 µl) were obtained by caudal puncture with a
heparinized 1 ml syringe (BD Syringe, Franklin Lakes, NJ, US) fitted with a
21-gauge needle and placed on ice; plasma samples were promptly obtained by
centrifugation (3 min at 10 000 g) (Eppendorf 5415D, Hamburg, Germany).
Following anesthesia in 0.2 g l–1 MS-222, fish were
immobilized and euthanized by cutting the spinal cord and piercing the brain,
and the gastrointestinal tract was subsequently exposed by dissection. Note
that this procedure rarely results in anal emptying when sampling occurs
immediately after euthanasia. The intestine was clamped immediately anterior
to the rectum and removed from the body cavity, after which the intestinal
contents were emptied into sample tubes for analysis, detailed below.
Gradual acclimation to low and high salinities
Groups of 6–8 toadfish were acclimated over a period of two weeks to
9, 35 and 50 ppt under static renewal conditions in tanks fitted with
biological filters and aeration. Natural seawater from Bear Cut is typically
35 ppt, while 9 and 50 ppt represent a lower and higher salinity tolerance of
cannulated toadfish. Water was changed every two days by siphoning off water
(80%) and detritus and replacing this volume with water of appropriate
salinity, either diluted or concentrated by addition of reverse osmosis water
or Instant Ocean sea salt, respectively, to acclimate fish to low and high
salinities. Salinities of the exposure waters were monitored by the use of a
refractometer, and resulting Na+, Cl–,
Mg2+ and SO42– were (in mmol
l–1): 112, 133, 12 and 5.3, respectively, for the 9 ppt
treatment; 454, 440, 46 and 24, respectively, for the 35 ppt treatment and
797, 649, 87 and 32 mmol l–1, respectively, for the 50 ppt
treatment. Fish were fed to satiation every two days; continued appetite was
considered an indication of acclimation with minimal stress. Measurements of
ammonia concentrations in water from the holding tanks revealed total
NH4+ concentrations of less than 112 µmol
l–1 in all cases.
Cannulation of acclimated toadfish
Following acclimation to 9, 35 and 50 ppt, toadfish were exposed to 0.2 g
l–1 MS-222 in the same salinity water to which they were
acclimated until anesthetized, and gills were perfused with 0.1 g
l–1 MS-222 in the appropriate salinity throughout surgery. A
caudal incision allowed for insertion of a catheter of polyethylene tubing
(PE50) (Intramedic, Becton Dickinson & Co., Sparks, MD, USA) into the
caudal artery or vein. The catheter was enclosed in a short sleeve of larger
tubing (PE160), the exposed segment of which was secured to the skin by silk
ligature, anchoring the catheter in the muscular tissue. The caudal incision
was treated with antibiotic (oxytetracyclin) before being closed with silk
ligatures. The catheter was filled with heparinized Hanks saline (50 i.u.
ml–1) (Walsh,
1987; Wilson and Grosell,
2003) and sealed. Each fish was also fitted with a rectal
collection sac consisting of a latex balloon securely tied to a 1 cm segment
of a 1 ml syringe (BD Syringe), heat-flared at both ends. The open end of the
syringe segment was inserted into the anus and held in place by a purse-string
ligature, allowing rectal contents to drain continuously into the balloon.
Immediately after surgery, fish were placed in individual flux chambers
containing a known volume (1 liter) of seawater at their acclimation
salinity. Following a recovery period, during which fish resumed their usual
activity level and behavior (10 min), initial water samples were taken
for analysis of ammonium and total titratable base. Fish were kept in these
aerated flux chambers for 24 h, at which point final water samples were
collected for 24 h flux measurements. The flux chambers were then flushed with
clean water of the appropriate salinity and a second 24 h flux was initiated.
At the end of this second 24 h flux, water samples were taken, blood was
sampled (200 µl) via the caudal catheter, and fish were
euthanized with an overdose of MS-222. The contents of the rectal sacs were
collected into pre-weighed 50 ml Falcon tubes, fish were weighed, and
intestinal contents (fluid and precipitate) were collected in pre-weighed 15
ml Falcon tubes as described above for the acutely transferred fish.
Analytical techniques
Intestinal and rectal samples were centrifuged to obtain solid matter, and
the fluid was transferred into separate pre-weighed sample tubes by pipetting.
The total amount of intestinal and rectal content and the proportions
represented by fluid and precipitate were determined by mass. Total
bicarbonate/carbonate content of intestinal precipitate was determined by
double-endpoint titration. Samples of precipitate isolated from rectal and
intestinal fluids were prepared for titration by homogenization and
resuspension in 5 ml deionized water. The prepared sample was continuously
aerated with N2 gas, titrated to pH 3.80 with 0.02 mol
l–1 HCl and then titrated back to the initial pH using 0.02
mol l–1 NaOH. For some precipitate samples, 0.2 mol
l–1 HCl and 0.02 mol l–1 NaOH were used in
order to minimize the volume of acid addition. The pH of the sample was
monitored using Ag/AgCl combination electrodes (Radiometer Analytical, PHC
3005-8, Lyon, France) and a pH meter (Radiometer, PHM201). Acid and base were
added using 2.0 ml micrometer syringes (GS-1200; Gilmont Instruments,
Barrington, IL, USA). In addition to analyzing ionic composition of the
intestinal and rectal fluids, the solutions resulting from the titrations of
rectal pellets were also analyzed for Mg2+ and Ca2+ to
determine the content of these ions in the rectal pellets. The fraction of
Mg2+ and Ca2+ eliminated from the rectum in precipitates
was calculated by relating the amount present in the pellets to the total
amount of these ions eliminated via fluids and pellets combined.
Double endpoint titrations were also done on initial and final water
samples (5 ml) from the flux chambers to determine total titratable acid flux
for each 24 h period. Blood plasma and intestinal fluids of cannulated
toadfish were analyzed for pH in contact with atmospheric air (Accumet
13-620-96 microelectrode; Fisher Scientific, Pittsburg, PA, USA; coupled to a
Radiometer PHM201 pH meter), and for total CO2 using a total
CO2 analyzer (Corning 965, Medfield, MA, USA). Anion concentrations
from all fluid samples were quantified by anion chromatography (Dionex 120,
Sunnyvale, CA, USA), while cations were analyzed by fast sequential flame
atomic absorption spectrometry (Varian 220, Palo Alto, CA, USA) using an
air/acetylene flame. Ammonium content of water samples was determined by
colorimetric assay (Verdouw et al.,
1978), modified for microplates using standards made up in
solutions of the appropriate salinity.
Bicarbonate equivalents in blood plasma, intestinal fluids and rectal
fluids for acclimated, cannulated fish were determined from the total
CO2 and pH measurements using the Henderson–Hasselbalch
equation. More specifically, the HCO3–
concentration was determined from Eqn
1 while the CO32– concentration was
determined from Eqn 2, in both
cases using a pKII of 9.46 for toadfish gut fluids
(Wilson et al., 2002):
 | (1) |
 | (2) |
). The HCO3– equivalents of
fluid samples measured in the present study were calculated as the sum of
[HCO3–] and
2x[CO32–]. Note that this approach has been
established previously, showing strong correlation between results obtained
from the above calculations and double endpoint titrations
(r2>0.999) (Grosell
et al., 1999). Extra intestinal fluxes of acid–base equivalents were determined from the change in water concentrations of titratable acid and total ammonia during the two subsequent 24 h periods, the volume of water in the flux chambers, the fish mass and the exact time elapsed. Rectal base output rates were determined from the total amount of base present in the excreted precipitates (determined by double endpoint titrations) and the total HCO3– equivalents in the excreted fluids (calculated from total CO2 and pH) at the end of the 48 h experimental period.
Data presentation and statistical analysis
All values are given as means ± s.e.m. The control (0 h
post-transfer in acutely transferred toadfish or 35 ppt in acclimated
toadfish) and experimental values were compared using Student's
t-tests with Bonferroni multi-sample comparison correction. Data sets
not found to be normally distributed were compared using Mann–Whitney
rank sum test. Differences between means were considered statistically
significant when P<0.05.
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RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Acute transfer to hypersalinity
Toadfish acutely transferred from 35 to 60 ppt displayed a transient
disturbance of acid–base balance. Total CO2 of both blood
plasma and intestinal fluids transiently increased immediately after salinity
transfer, followed by a significant reduction in plasma total CO2
at 96 h post-transfer (Fig. 1).
In the intestinal fluid, Cl– concentration was elevated at
both 24 and 96 h post-transfer (Fig.
2), which coincides with the decrease to initial values seen in
total CO2 in the intestinal fluid at these time points
(Fig. 1). By contrast,
Na+, Ca2+, K+ and
SO42– concentrations in the intestinal fluids were
relatively stable over time. However, in the plasma of toadfish transferred
acutely to 60 ppt (Fig. 3),
both Na+ and Cl– increased during the first 24 h
after transfer, while Ca2+ was significantly lower than control
values after 96 h (P<0.03) and the concentration of K+
increased greatly in the first 24 h, returning to initial levels by 96 h. The
low plasma Mg2+ concentrations remained constant
(Fig. 3) following transfer to
60 ppt.
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Gradual acclimation to low and high salinities
Plasma HCO3– equivalents in toadfish acclimated
to both 9 ppt and 50 ppt were not significantly different from those of
samples obtained from toadfish in 35 ppt. Bicarbonate equivalents in the
rectal fluid are relatively constant in all salinities
(Fig. 4). Rectal fluid pH was
alkaline in all samples but was significantly decreased in 50 ppt samples and
increased in isosmotic conditions (9 ppt) compared with control values (35
ppt). Similarly, plasma pH was lower at 50 ppt and higher at 9 ppt compared
with 35 ppt. Note that plasma samples reflect the status of the animals at the
48 h time point whereas rectal fluid was accumulated over the entire 48 h
period.
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All measured ions in the plasma (Na+, Cl–, Mg2+, Ca2+, K+) tended to be higher in 50 ppt than in 35 ppt (Table 1), although none of these differences was statistically significant. In the rectal fluid of acclimated toadfish (Table 2), the concentrations of K+ and Na+ decreased from 9 to 35 ppt whereas SO42– increased. Similarly, Mg2+ greatly increased both from 9 to 35 ppt, and from 35 to 50 ppt. The absolute ion excretion rate (µmol kg–1 h–1) from the rectum over 48 h is shown in Fig. 5. In toadfish acclimated to 50 ppt, Mg2+ and Cl– excretion was significantly greater than in 35 ppt, with a similar, but not statistically significant, trend for SO42–, Na+, K+ and Ca2+. Intestinal excretion of HCO3–, Ca2+ and Mg2+ occurs both in solution and via precipitated solids. The amount of both Ca2+ and Mg2+ excreted as both fluid and precipitate increased with increasing salinity (Fig. 5). The fraction of Ca2+ excreted as precipitate increased from 26.8% in 35 ppt to 61.2% in 50 ppt fish, while the percentage of excreted Mg2+ in the precipitate was very low (2.7% in 35 ppt and 3.6% in 50 ppt). Rectal base excretion, as both HCO3– equivalents in rectal fluids and CO32– precipitates, increased with salinity, and the fraction of rectal base efflux occurring as precipitate increased from 16.7% in 35 ppt to 23.4% in 50 ppt fish (Fig. 6). Extra-intestinal net acid excretion (sum of titratable acid flux and total ammonia flux) also increased with increasing salinity (Fig. 6). Interestingly, total ammonia excretion in itself tended to increase with increasing salinity (P<0.062).
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DISCUSSION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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).
Our results suggest that free-swimming, non-cannulated gulf toadfish can
maintain normal regulation of plasma ionic composition in 60 ppt for at least
96 h. However, a preliminary experiment in which fish were acclimated to 60
ppt and underwent cannulation surgery resulted in high mortality. The
acclimation salinity was therefore decreased to 50 ppt for completion of
cannulation experiments in the present study.
Increased drinking rate in elevated salinity
It is well-established that drinking rates of teleost fish increase with
increased salinity (Shehadeh and Gordon,
1969; Sardella et al.,
2004; Marshall and Grosell,
2005). Fish in hypo- or isosmotic salinities have little need for
water absorption across the gastrointestinal tract. Thus, as expected, the
drinking rate of toadfish in isosmotic conditions is low, demonstrated by the
low rate of fluid excretion from the rectum at 9 ppt compared with secretion
rates from fish in 35 and 50 ppt. Drinking rates were not determined directly
in the present study in fish fitted with rectal catheters but can be estimated
from the volume of rectal fluid collected and the concentrations of
Mg2+ and SO42– in these fluids and in
the ambient water. Such estimates rely on the assumption that the intestinal
epithelium is relatively impermeable to MgSO4 with little, if any,
absorbed by the intestine. This has been demonstrated previously
(Hickman, 1968) and also is
supported by recent findings of very low MgSO4 absorption rates by
isolated toadfish intestinal segments
(Grosell and Taylor, 2007).
Based on the concentration of Mg2+ in the rectal fluid, the volume
of rectal fluid excreted, and measured Mg2+ concentrations from all
experimental salinities, we calculated drinking rates of 0.98±0.42,
2.56±0.87 and 3.75±0.59 ml kg–1
h–1 at 9, 35 and 50 ppt, respectively. Corresponding
estimates based on rectal concentrations of SO42–
and measured ambient SO42– concentrations are
1.79±0.55 (9 ppt), 2.63±0.97 (35 ppt) and 3.89±0.57 ml
kg–1 h–1 (50 ppt). Considering these
observations of Mg2+ and SO42–
combined, drinking rates can be estimated to be 1.38±0.30,
2.60±0.92 and 3.82±0.58 ml kg–1
h–1 in 9, 35 and 50 ppt, respectively. No significant
differences exist between the drinking rate estimates based on concentration
of Mg2+ versus SO42–, but
drinking rates at 50 ppt were significantly higher than at 9 ppt according to
both estimation methods. The mean estimated drinking rate based on rectal
fluid excretion (of both Mg2+ and
SO42–) in 50 ppt is not significantly different
from that directly measured in non-cannulated toadfish acclimated to 50 ppt
(3.82±0.58 ml kg–1 h–1 compared with
3.24±0.34 ml kg–1 h–1, respectively).
The measured rate at 50 ppt is higher than the mean rate estimated for
cannulated fish in 35 ppt (2.60±0.92 ml kg–1
h–1) and higher than those previously reported for toadfish
acclimated to 30 ppt (Grosell et al.,
2004). Admittedly, if MgSO4 was absorbed by the
intestine, our calculations would have underestimated the actual drinking
rate. However, we note that our estimated drinking rates are well within the
range established for seawater fish (reviewed by
Marshall and Grosell, 2005)
and that measured and estimated drinking rates for the 50 ppt fish are
similar.
It is known that cortisol, a key stress hormone, has a role in the
regulation of drinking rate in teleost fish
(Fuentes et al., 1996;
Lin et al., 2000). Although
transfer to higher salinity increases drinking rate, simultaneous addition of
cortisol increases drinking rate to an even greater extent in both tilapia
larvae (Lin et al., 2000) and
juvenile rainbow trout (Fuentes et al.,
1996). The estimated drinking rates for cannulated toadfish may
thus be higher than those measured in non-cannulated fish due to the
combination of high salinity and stress from handling and extensive surgical
procedures.
Fractional fluid absorption
The difference between the estimated drinking rate (over 48 h) and the
measured rectal fluid excretion yields an estimate of total fluid absorption
by the gut (Fig. 7). In fish
acclimated to 35 ppt, 68.8±3.2% (1.90±0.74 ml
kg–1 h–1) of the ingested seawater is
absorbed by the gastrointestinal tract, which is within the range for seawater
fish determined previously, which includes 38.5%
(Wilson et al., 2002), 75.8%
(Hickman, 1968), 80%
(Shehadeh and Gordon, 1969)
and 84.9% (Wilson et al.,
1996). Absorption values over the 48 h flux period were also
estimated for toadfish in 9 ppt (1.21±0.27 ml kg–1
h–1) and 50 ppt (2.36±0.36 ml kg–1
h–1) to be 85.9% and 61.4% of the ingested volume,
respectively. It is apparent that intestinal fluids in high salinity are
depleted of NaCl, while MgSO4 is concentrated to very high levels
(Table 2). As mentioned
previously, the intestinal epithelium has very low permeability to
Mg2+ and SO42–
(Grosell and Taylor, 2007).
Therefore, as salinity increases and permeable salts are absorbed, the
dominant cation in the gastrointestinal fluids shifts from Na+ to
Mg2+ while the dominant anion shifts from Cl– to
SO42– and HCO3–. As
the ions available to drive water absorption are taken up by the epithelium
and impermeable ions accumulate, it becomes increasingly difficult to absorb
water from the concentrated fluid in the lumen. This point is illustrated in
Fig. 8, which displays the
absorption rate of ingested Na+ and Cl– as well as
the fractional absorption of these ions. Absorption of these ions dramatically
increases with salinity, although fractional absorption does not increase from
35 to 50 ppt, apparently because fractional water absorption at 35 ppt has
already reached a maximum. The limitation of water absorption by extensive
removal of Na+ and Cl– and increased concentration
of impermeable, divalent ions in the intestinal fluids likely explains the
observed decrease in the fraction of ingested water that is absorbed by the
gastrointestinal tract with increasing salinity. It thus appears that, since
fractional water and NaCl absorption cannot increase at salinities higher than
35 ppt, the only mode of response to the elevated diffusive fluid loss is
increased drinking rate, as was observed in the present study.
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Acid–base response to elevated salinity
Rectal HCO3– equivalent excretion is higher in
toadfish acclimated to 50 ppt than to 35 ppt, indicating increased intestinal
HCO3– secretion in response to increased drinking
rate and osmoregulatory demand. Total base excretion increased with salinity,
as did the proportion occurring as precipitate (3.3%, 16.7% and 23.4% at 9, 35
and 50 ppt, respectively). Consistent with this observation, plasma pH is
significantly lower in toadfish acclimated to 50 ppt than in 35 ppt-acclimated
fish, indicating an acid–base balance disturbance caused by increased
HCO3– secretion into the intestinal lumen in
response to elevated salinity. The mechanism for apical transport of
HCO3– in the intestinal epithelium has been
characterized and shown to occur in parallel with H+ transport
across the basolateral membrane in gulf toadfish
(Grosell and Genz, 2006).
Thus, when these transport processes occur to a greater extent in high
salinity, an elevated net acid load in the extracellular fluids occurs.
However, the acid–base disturbance observed in toadfish acclimated to 50
ppt is much less dramatic than could be expected given the intensity of the
osmoregulatory challenge and the 21-fold increase in total rectal base efflux
between 9 ppt (9.3±2.7 µmol kg–1
h–1) and 50 ppt (193.2±64.9 µmol
kg–1 h–1). The limited nature of the
whole-animal acid–base balance disturbance (modest changes in
HCO3– equivalents and pH in extracellular fluids)
is explained by adjustments occurring on the whole-animal scale, which include
markedly elevated extra-intestinal net acid excretion to maintain
acid–base balance following salinity transfer
(Fig. 6C). We note that our
plasma pH values (8.06) are higher than values previously reported (7.85)
from toadfish in seawater (Barber and
Walsh, 1993), a difference we ascribe to our plasma pH
measurements not being performed under gastight conditions. To evaluate this
potential influence of diffusive CO2 loss from samples exposed to
atmospheric air prior to pH measurements, additional measurements were
performed. Blood obtained via Hamilton syringes from toadfish
(N=5) fitted with caudal catheters was analyzed immediately for pH in
a custom-made gastight, water-jacketed chamber fitted with a Radiometer
combination pH electrode (4000-8). Subsequently, a fraction of these
individual blood samples was subjected to the procedure used for the above
analysis, and plasma pH was measured under contact with atmospheric air. The
pH values obtained using gastight measurements on whole blood were
7.824±0.045, while the values obtained from air-exposed plasma for a
time period relevant to the original measurements were 7.992±0.027.
These follow-up measurements thus suggest that air exposure of the plasma
samples accounts, at least in part, for the relatively high pH values obtained
in the present study. However, samples from all experimental groups were
treated the same, such that differences among experimental groups should be
robust.
Gill and kidney as possible sites of compensatory acid excretion
The gill is the primary organ responsible for regulation of acid–base
balance in teleost fish. Another possible route for extra-intestinal acid
excretion is the kidney. However, in the aglomerular toadfish, the kidney
plays a modest regulatory role, even less so than the limited impact observed
in glomerular fish (McDonald et al.,
1982; Maren et al.,
1992). Titratable acid fluxes determined as part of the present
study demonstrate an increase in extra-intestinal, presumably branchial, net
acid excretion in elevated salinity (Fig.
6). Thus, it seems that increased acid extrusion at the gill
compensates for increased transport of H+ into the extracellular
fluids occurring in response to intestinal processes associated with high
salinity. Further studies of the dynamics of this compensatory branchial acid
excretion, and the underlying mechanisms, are clearly warranted.
Nitrogenous waste excretion at the gill
Just as the gill extruded more H+ in elevated salinity,
branchial NH4+ (or NH3) excretion also
appeared to be elevated. Under normal conditions, toadfish excrete nitrogenous
waste primarily as ammonia (McDonald et
al., 2006). During periods of acute stress, however, nitrogenous
waste excretion shifts to favor urea
(Hopkins et al., 1995). The
increased NH3/NH4+ excretion observed in this
study is contrary to what would be expected in stressed and confined toadfish
and is therefore unlikely to be related directly to osmoregulatory and
surgery-related stress and may instead represent a response to the
acid–base balance disturbance or the excess energy demand associated
with an increased osmotic challenge. It has previously been observed that urea
production decreases during hypercapnia
(Barber and Walsh, 1993;
McDonald et al., 2007).
Increased intestinal HCO3– secretion in high
salinity diminishes HCO3– concentration in
extracellular fluids and it is clear that an osmoregulation-related acidosis,
although modest, occurs in high salinity. It is plausible that the observed
increase in branchial NH3/NH4+ secretion may
be a compensatory mechanism for regulation of acid–base balance. An
increase in NH4+ rather than NH3 excretion
would be advantageous for maintenance of acid–base balance by serving
the dual function of both acid excretion (as NH4+) and
the retention of HCO3–, which would otherwise be
consumed during urea production (Atkinson,
1992). Excretion of NH4+ rather than
incorporation of nitrogen into urea would allow adequate excretion of
nitrogenous waste and would contribute to the correction of acid–base
balance. Furthermore, it might act as a mechanism for energy retention, as
urea synthesis is an ATP-consuming process. It is generally assumed that
nitrogenous waste excretion by ammoniotelic marine teleosts occurs
via a paracellular route and that it is driven mainly by the
blood-side positive transepithelial potential (TEP)
(Wilkie, 2002). However, the
experimental evidence for this assumption is circumstantial at best and it
cannot be dismissed that NH3 excretion occurs, especially since the
gulf toadfish displays a blood-side negative TEP in seawater
(Evans, 1980). In contrast to
NH4+, excretion of NH3 would not confer an
acid–base balance advantage during exposure to hypersalinity but would
rather contribute to the acidosis arising from intestinal transport processes.
The argument for energy conservation obtained by excretion of
NH3/NH4+ rather than the metabolically
expensive urea relies on the assumption that the metabolic cost of ammonia
excretion is negligible compared with the cost of urea synthesis and
excretion. Despite significant progress in the understanding of urea excretion
by the gulf toadfish (McDonald et al.,
2006), the metabolic cost remains unknown. Similarly, the rapidly
developing field of NH3/NH4+ excretion by
fish (Nawata et al., 2007;
Hung et al., 2007;
Nakada et al., 2007) still
lacks insight into the energetic driving force and thus the metabolic cost.
Unfortunately, urea excretion was not measured as part of the present study
but, considering the observed NH3/NH4+
excretion increase, the above discussion is relevant in the case of unaltered
or reduced urea excretion and we can infer an apparent impact of intestinal
osmoregulatory processes on branchial nitrogenous waste excretion. To our
knowledge, this is the first report of increased
NH3/NH4+ excretion at the gill being linked
to a hyperosmoregulatory challenge. Directly investigating this connection
between salinity, acid–base balance and the mode of nitrogenous waste
excretion is an exciting area for future work.
Conclusions and future directions
It is generally acknowledged that most teleost fish display an acidosis and
decreased HCO3– equivalents in the blood plasma
upon transfer from freshwater to seawater
(Wilkes and McMahon, 1986;
Nonnotte and Truchot, 1990;
Maxime et al., 1991), a
phenomenon also observed in this study following transfer to elevated
salinity. Concentrations of Cl– and Na+ determined
in this study also agree with previous work
(Bath and Eddy, 1979;
Wilkes and McMahon, 1986;
Maxime et al., 1991), with
both ions increasing in the plasma over the first 24 h post-transfer, and
absorption of Cl– into the extracellular fluids increasing to
a greater extent than Na+ (Table
1, Fig. 8).
Overall, we conclude that increased intestinal
HCO3– secretion in elevated salinity in the gulf
toadfish creates an acid–base balance disturbance, which is rapidly and
almost completely corrected by increased branchial H+ excretion.
These two processes offer an explanation for the commonly observed (transient)
acidosis following transfer to hypersalinity. To our knowledge, this is the
first demonstration of intestinal transport processes involved in
osmoregulation having an impact on acid–base balance, as well as net
acid extrusion and NH3/NH4+ excretion at the
gill. Our observations add to the accepted role of NaCl excretion at the gill
compensating for intestinal NaCl absorption, illustrating how these two organs
operate in concert to maintain not only salt and water balance but also
acid–base homeostasis. Increased excretion of
NH3/NH4+, in response to the acid–base
disturbance in high salinity, suggests an additional and unique connection
between osmoregulation and excretion of nitrogenous waste. The role of the
kidney on acid–base balance with regards to physiological demands of
salinity transfer has previously been investigated and found to be relatively
minimal, particularly in aglomerular fish such as O. beta, but it
would be worthwhile performing integrative experiments to clarify how the
renal processes might be related to the salinity response observed in the
present study.
The extent to which intestinal osmoregulation impacts acid–base
balance and the importance of other organs, notably the gill, in compensating
for acid–base disturbances in high salinity may be variable among
species. Species that naturally see large, rapid salinity fluctuations due to
tidal movements would be predicted to have faster, more efficient adjustment
mechanisms for osmoregulation and maintenance of acid–base balance when
presented with a salinity challenge, and could be promising candidates for
future work in this area. However, such species may continuously possess
osmoregulatory and acid–base balance mechanisms to accommodate a range
of salinities. Fish that rarely see fluctuations in salinity (i.e. anadromous
species such as many salmonids) may offer insight into the cellular mechanisms
regulating water, ion and acid–base balance, particularly at the
transcriptional level, as these mechanisms would likely be recruited during
environmental challenges associated with salinity change. Examples of this for
gill tissue are ample in the current literature
(Marshall and Grosell,
2005).
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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7). An asterisk (*) indicates statistically
significant difference from 0 h value (P<0.05).
