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First published online November 30, 2007
Journal of Experimental Biology 210, 4359-4367 (2007)
Published by The Company of Biologists 2007
doi: 10.1242/jeb.010694
Strategies for regulation of hemolymph pH in acidic and alkaline water by the larval mosquito Aedes aegypti (L.) (Diptera; Culicidae)
Indiana University South Bend, South Bend, IN 46615, USA
* Author for correspondence (e-mail: tclark2{at}iusb.edu)
Accepted 27 September 2007
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Summary |
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Key words: hemolymph pH, pH homeostasis, Malpighian tubules, rectum, mitochondrial density, mosquito, larva, Aedes aegypti
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Introduction |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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).
pH is thus an extremely important physical factor limiting the distribution
and abundance of aquatic animals. Larval mosquitoes are remarkably tolerant of
extreme pH, allowing them to exploit a wide variety of habitats in nature
(Clements, 2000;
Clark et al., 2004). Larvae of
the mosquitoes Aedes aegypti and Ochlerotatus taeniorhynchus
complete development in waters ranging from pH 4 to pH 11 in the laboratory.
Across this range, hemolymph pH of acclimated larvae varies by only 0.1 pH
units or less (Clark et al.,
2004). They show phenotypic plasticity in pH tolerance in which
acclimation to pH 4 or 11 increases their ability to tolerate subsequent
exposure to more extreme pH (i.e. pH 3 or 12, respectively).
In larval endopterygotes, pH is regulated in two major extracellular
compartments, the hemolymph and the midgut lumen. The cellular mechanisms
involved in the generation of highly alkaline conditions within the midgut of
lepidopteran and mosquito larvae have received considerable attention. In
contrast, the physiology of acid–base homeostasis of insect hemolymph
continues to be a neglected area of study. In fact, the specific contributions
of each organ of the alimentary and excretory systems to elimination of a
hemolymph acid or base challenge are known only for a single insect, the
locust S. gregaria. In the locust, an acid load injected into the
hemocoel was cleared primarily by the hindgut. The Malpighian tubules secreted
acidic fluid, but their contributions to acid–base homeostasis were
minor (Harrison et al., 1992;
Stagg et al., 1991;
Phillips et al., 1993;
Harrison, 2001). Responses of
locusts to alkaline challenges have not been described. Little is known about
the regulation of hemolymph pH in other insects
(Cooper, 1994;
Harrison, 2001).
Aquatic insects rely primarily on epithelial transport across renal systems
for acid–base homeostasis (Cooper,
1994; Harrison,
2001). The ion transport mechanisms relevant to acid–base
homeostasis are expected to be located in ion-transporting epithelia including
the midgut, the renal system (consisting of the Malpighian tubules and
hindgut) and extrarenal ion-transporting organs. The Malpighian tubules form
the primary urine, while the rectum recovers water and ions as necessary, and
secretes additional ions. Aquatic insects frequently possess extrarenal organs
such as anal papillae (AP), or clusters of mitochondria-rich chloride cells,
that provide increased surface area for mechanisms involved in ionic
homeostasis (Komnick et al.,
1972). The Malpighian tubules and hindgut of Ochlerotatus
taeniorhynchus possess inducible specific transport mechanisms for
secretion of a variety of ions (Bradley and
Phillips, 1977; Maddrell and
Phillips, 1978). Most inducible ion transport systems are located
in the rectum, with the exception of inducible
SO42– transport, which occurs in the Malpighian
tubules (Maddrell and Phillips,
1978). Induction of H+ transport was not
investigated.
The limited work on larval mosquito hemolymph pH homeostasis in alkaline
media emphasizes the role of the rectum. Larvae of the mosquito Aedes
dorsalis inhabit alkaline lakes containing high concentrations of
bicarbonate, and under these conditions bicarbonate is excreted into the
rectum via HCO3–/Cl–
exchange (Strange and Phillips,
1984; Strange et al.,
1982; Strange et al.,
1984). The AP of larval mosquitoes and related Diptera consist of
four elongated gill-like structures attached to the last abdominal segment.
They are covered with cuticle, contain a cellular syncetium, and can be
isolated from the hemolymph by the actions of a ring of muscles at their base
(Clements, 2000). The AP of
larval mosquitoes are known to be important sites of ion uptake, and are the
region of the cuticle most permeant to water
(Wigglesworth, 1933;
Wigglesworth, 1938;
Koch, 1938). Larval Aedes
aegypti reared in dilute water have larger AP
(Wigglesworth, 1938), with
greater mitochondrial densities (Edwards
and Harrison, 1983), than larvae from less dilute media. These
increases have been attributed to increased energetic requirements for active
uptake of NaCl from the medium (Koch,
1938; Wigglesworth,
1938; Edwards and Harrison,
1983). The role of these organs in acid–base balance has not
been investigated. Mechanisms used by larval mosquitoes to maintain hemolymph
pH homeostasis in acidic media have not been addressed.
In the present study, responses of larval Aedes aegypti to acidic (pH 4), neutral and alkaline (pH 11) media allowed the elucidation of the overall physiological strategies of hemolymph pH homeostasis in this insect. This study focused on the roles of the Malpighian tubules, rectum and AP in the regulation of hemolymph pH. Evidence suggests that the larvae utilize novel and unexpected regulatory strategies to maintain homeostasis at each end of the tolerable pH range. It appears that the Malpighian tubules play a major role in acid excretion in acidic media. No evidence was obtained for an active role of any organ in acid–base homeostasis during alkaline challenges.
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Materials and methods |
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). This
allowed the observed physiological changes to be attributed with greater
certainty to differences in pH. In the present study, rearing solutions low in
NaCl were also prepared at pH 4, 7 and 11 (low-NaCl RS 4, 7 and 11). These
low-NaCl RS contained the same buffers, and were adjusted to pH in the same
way, but any NaCl present consisted only of that present in the food and the
Na+ or Cl– added while adjusting the pH of the
solution.
Mitochondrial luminosity
To isolate Malpighian tubules, the head and seventh abdominal segment of
late-stage fourth instar larvae were severed under cold mosquito hemolymph
substitute solution (HSS) (Clark et al.,
2005). Fine forceps were then used to grasp the esophagus or the
gastric caeca and pull the gut from the body using care to avoid stretching
the tissue. To label mitochondria, guts with attached Malpighian tubules and
terminal segments with AP were incubated for 30 min in cold HSS containing 50
nmol l–1 Mitotracker Green FM (Molecular Probes Inc., Eugene,
OR, USA). They were then placed on a coverslip with a drop of glycerol.
Mitotracker Green FM only fluoresces when bound to a mitochondrial membrane,
and does not require respiring mitochondria (product literature, Molecular
Probes Inc.). Mitotracker Green fluorescence was then recorded in whole mounts
using a Zeiss Axioskop microscope (Oberkochen, Germany), with a Kubler Codex
ebq100 lamp source (Gena, Germany). The excitation and emission wavelengths of
Mitotracker Green are 490 and 516 nm respectively; an Omega Optical XF100-2
filter set (Brattleboro, VT, USA) was used. Images were captured at x100
magnification using a Pixera Penguin 150CL digital camera (Los Gatos, CA, USA)
under manual control (exposure 1/8 s). Because the same exposure time and
magnification were used for all images, it was possible to quantify changes in
the mitochondrial signature of the tissues. Images were imported into Adobe
Photoshop where luminosity was quantified from the intensity of the
fluorescence in boxes of uniform pixel numbers.
Drinking rates
The rates at which acclimated larvae drink RS were determined at each pH by
placing larvae in 1 ml of their respective RS containing 0.5 g
l–1 fluorescein isothiocyanate conjugated to dextran
(FITC-dextran, average molecular mass 4.3 kDa; Sigma) for a period of between
1 and 3 h. The treatment groups were sampled in repeated series during assays
to avoid artifacts from possible time-dependent changes in drinking rates.
Controls consisted of larvae ligated at the neck, and assayed alongside
treatment groups at each pH. Following exposure to FITC-dextran, larvae were
rinsed, blotted dry, weighed to the nearest 10 µg, and homogenized in 200
µl of cold Tris-buffered saline. This step ensured that the fluorescence of
FITC-dextran was always determined at the same final pH. Following
centrifugation for 1 min at 18 000 g, the fluorescence of the
supernatant was quantified in a Turner Designs TD-700 Fluorometer with
minicell adaptor (Sunnyvale, CA, USA). The FITC-dextran content of each larva
was determined by comparison with a standard curve. The fluorescence of
ligated controls, due to a combination of autofluorescence and low rates of
transcuticular FITC-dextran entry, was subtracted from treatment values
assayed at the same pH. This corrected for possible artifacts such as effects
of pH on transcuticular FITC-dextran permeability.
Effects of pH challenges on total body water
The effects on total body water of the transfer of acclimated larvae to
more acidic media were determined in the presence and absence of NaCl. Tests
performed in the presence of NaCl involved rearing larvae in RS 7 or RS 4.
Fourth instar larvae were then either maintained at the rearing pH or
transferred to RS 3 for 2 h. In similar experiments without NaCl, larvae
reared in low-NaCl RS 7 were assayed in either low-NaCl RS 7 or low-NaCl RS 3.
Following exposure, larvae were blotted dry, and wet mass was determined to
the nearest 1x10–5 g using a Mettler-Toledo AX205
deltarange balance (Columbus, OH, USA). The larvae were then dried overnight
in a drying oven at 96°C, and reweighed. The decrease in mass represents
total free body water while the ratio of body water to total mass represents
the percentage body water or body water ratio, calculated as: [(wet mass
– dry mass)/wet mass].
pH of the rectum in vivo
Larvae reared in RS 4, 7 and 11 were exposed to kaolin and azolitmin (1 g
per 50 ml) for 24 h. Kaolin is an inert silicate that is ingested by larvae,
displacing the food column and providing a background against which the color
of ingested pH indicators can be established
(Dadd, 1975). They were then
transferred to RS 4, 7 or 11. Each combination of rearing and acute pH
exposure was performed. The larvae were photographed after 24 h of exposure to
the assay pH using an Olympus C-3040 digital camera through a Leica Stereozoom
6 microscope (Wetzlar, Germany).
pH of the AP in vivo
It was noted that bromothymol blue enters the AP in acidic media allowing
the investigation of the acid–base permeability of the AP. Bromothymol
blue was initially dissolved in dimethyl sulfoxide (7.6 mg per 10 ml). This
mixture was vortexed, then centrifuged. The supernatant was diluted 1:1000 in
RS 4. Larvae were exposed to this solution for 24 h. They were then placed
into RS lacking bromothymol blue. The pH of the AP was noted, and the larvae
were photographed within 5 min and at 24 h of exposure to the assay pH using
an Olympus C-3040 digital camera through a Leica Stereozoom 6 microscope.
Bromothymol blue was also visible in the rectum of several of these larvae
allowing confirmation of the azolitmin results.
Morphology of the AP
Lengths of AP were determined for larvae reared in RS 4, 7 and 11, in
low-NaCl RS 4, 7 and 11, and in deionized water, 5.25 g l–1
artificial seawater and 10.5 g l–1 artificial seawater
(Instant Ocean, filtered; Aquarium Systems, Mentor, OH, USA). Lengths of AP of
larvae fixed in 2% glutaraldehyde in PBS were determined with a Leica
Stereozoom 6 with ocular micrometer. Larvae were oven dried for 24 h at
96°C, then weighed to the nearest 1x10–5 g in order
to determine the mass-specific length of the AP.
Rates of acid–base excretion
Larval acid–base excretion rates were determined under controlled
conditions by rinsing fed, acclimated larvae twice in fresh RS, and placing
them individually into 2.0 ml of fresh RS 4 or RS 11. RS aliquots without
larvae were run alongside larvae and served as paired negative controls. After
a period of 1–2 h, the pH of the experimental and control solutions was
determined. Titration of the RS allowed calculation of the rate of acid
excretion from the difference in pH of the experimental and control
solutions.
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;
Clements, 2000). The presence
or absence of NaCl did not influence the effect of pH on drinking rates
[P>0.05, single factor ANOVA followed by
Student–Newman–Keuls (SNK) a posteriori test with
=0.05].
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=0.05) (Sokal and Rohlf,
1969). Total body water was reduced in larvae reared in RS 4
relative to RS 7. Total body water increased when larvae reared in RS 4 were
transferred to RS 3, and when larvae reared in RS 7 or low-NaCl RS 7 were
transferred to RS 3 or low-NaCl RS 3, respectively. Because chronic exposure
to acidic water resulted in increased drinking rates, but decreased percentage
body water, fluid excretion rates must increase as well. In the presence of
NaCl, fluid ingestion and excretion rates in acidic water (pH 4) were
approximately 20 times those in alkaline water (pH 11; 5.9 vs 0.3 ml
g–1 day–1). In the absence of NaCl, they
were 7.9-fold greater in acidic water than in alkaline water (7.1 vs
0.9 ml g–1 day–1). Drinking rates were
similar in neutral and alkaline media and in the presence and absence of NaCl
(Fig. 1).
Effects of ambient pH on acid–base excretion
Larvae in RS 4 did not change the pH relative to controls over 1–2 h
time intervals. Larvae in RS 11 excreted net acid (0.12±0.017 nequiv
g–1 h–1, mean ± s.e.m.) relative to
paired larva-free controls (larvae vs larva-free controls,
P<1x10–9, two-factor ANOVA without
replication, EXCEL).
Effects of ambient pH on mitochondria
Changes are observed in the fluorescence of the mitochondrial dye
Mitotracker Green FM in response to chronic pH exposure. Mitochondrial
luminosity was higher in both proximal and distal Malpighian tubule regions of
animals reared in acidic water than in larvae reared in neutral or alkaline
media, which did not differ in luminosity
(Fig. 2; proximal tubule:
P<0.05, F=4.24, d.f.=17; distal tubule:
P<0.005, F=8.92, d.f.=17; followed by SNK)
(Sokal and Rohlf, 1969). In
larvae reared in acidic media (RS 4), the distal Malpighian tubule showed
significantly greater luminosity than the proximal region (P<0.05,
two-tailed, paired Student's t-test, N=6 tubules). No
differences in luminosity were observed within pH between proximal and distal
regions of the Malpighian tubules of larvae reared in RS 7 or RS 11 (RS 7,
P>0.5; RS 11, P>0.09, two-tailed, paired
t-test, N=6 tubules/RS). The influence of pH on hindgut
mitochondrial luminosity was not determined due to difficulties experienced in
the removal of the rectal contents, which autofluoresce.
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Mitotracker Green FM produced uneven fluorescence within the AP. Luminosity was always greatest in the proximal and distal regions, and lowest in the central region (Fig. 3; by region, pH 4: P<0.0001, F=12.646, d.f.=65; pH 7: P<0.01, F=5.137, d.f.=56; pH 11: P<0.0005, F=8.777, d.f.=62; single factor ANOVA followed by SNK). Changes were observed in Mitotracker Green FM fluorescence, within the AP, in response to chronic pH exposure. Animals reared in RS 4 showed reduced luminosity across regions compared with animals reared in RS 7 or 11 (Fig. 3; P<0.05, F=3.161, d.f.=61, single factor ANOVA followed by SNK.
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The pH of the rectal lumen
The pH indicator azolitmin revealed that larvae always have an acidic
rectal lumen (pH <6.2), even when chronically exposed to RS 11
(Fig. 4; N=12 each in
RS 4, RS 7 and RS 11). Similar results were obtained using bromothymol blue
(transition from yellow to blue at pH 6.8;
Fig. 5). Obtaining similar
results with two separate pH indicators provides increased confidence that the
excretory system of larvae exposed to highly alkaline media eliminates fluid
more acidic than the hemolymph.
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Effects of salinity and ambient pH on larval mass and the size of the AP
The size of AP is influenced by ambient salinity and by pH (Figs
6 and
7). The AP were longest in
dilute water, and length decreased with salinity
(Fig. 6A; P<0.05,
F=3.97, d.f.=25, single factor ANOVA). The dry mass of larvae used to
determine the effects of environmental conditions on the length of AP differed
in both the salinity and pH experiments. Significant differences in dry mass
were recorded among salinities (P<0.05, F=4.66, d.f.=25).
Among media differing in pH values, significant differences were recorded in
the presence of NaCl (P<0.0005, F=11.25, d.f.=29) but not
in the absence of NaCl (P>0.21, F=1.64, d.f.=29;
Table 1). However, because
salinity also influences mass, the mass-specific lengths of the AP were also
determined. No differences were observed in mass-specific lengths (mm
mg–1 dry mass) of the AP across salinities
(Fig. 6B; P>0.27,
F=1.37, d.f.=25, single factor ANOVA) although larvae reared at the
highest salinities possessed the smallest AP.
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In contrast to salinity, pH influenced both the length and mass-specific length of the AP of larvae reared in RS containing 59.9 mol l–1 NaCl (Fig. 7A,B; length: P<0.01, F=6.96, d.f.=29; mass specific length: P<0.0001, F=15.34, d.f.=29, 2-way P values, single factor ANOVA). Under these conditions, the AP of larvae reared in RS 4 were reduced in both length and mass-specific length relative to those reared in RS 7, while those reared in RS 11 possessed the longest AP. The decrease in mass-specific length in acidic media was proportionally much greater than the decrease in length. In contrast, pH had no effect on the length, or mass-specific length, of the AP of larvae reared in low-NaCl RS (Fig. 7A,B; length: P>0.27, F=1.39, d.f.=29; mass-specific length: P>0.87, F=0.14, d.f.=29, 2-way P values, single factor ANOVA).
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The role of the Malpighian tubules in acid–base homeostasis
The Malpighian tubules appear to be primarily responsible for
acid–base homeostasis in acidic media. During exposure to acidic media,
larvae increased drinking rates substantially. Naïve larvae became volume
loaded whereas acclimated larvae maintained high drinking rates yet showed
reduced body water. Exposure to acidic media thus results in increased rates
of fluid flux through the organism. Acclimation to acidic media also resulted
in an increase in fluorescence of a mitochondria-specific dye in the
Malpighian tubules. The increase in Malpighian tubule mitochondria is
presumably paralleled by upregulation of specific transport mechanisms driving
increased rates of fluid secretion.
We have not yet established the pH of the fluid produced by the larval
Malpighian tubules, or whether the pH of the secreted fluid changes during
acid exposure. However, it is not necessary for the H+
concentration or buffer capacity of the excreted fluid to increase for overall
Malpighian tubule H+ excretion rates to increase, if the volume of
secreted fluid increases. Malpighian tubules of adult A. aegypti
secrete acidic fluid, and cyclic AMP increases the rate of fluid secretion
while pH remains constant, resulting in elevated H+ clearance rates
(Petzel et al., 1999). The
transport mechanisms of larval and adult Malpighian tubules differ
(Clark and Bradley, 1996),
however, and it remains to be determined whether the larval Malpighian tubules
respond in a similar way during acid exposure. We also do not rule out an
additional increase in H+ excretion rates due to an increase in
secretion of buffer or ammonia during acid challenges, as occurs in the
mammalian kidney.
The role of the rectum in acid–base homeostasis
Evidence presented here suggests that the role of the larval mosquito
rectum in alkaline media should be re-evaluated. A series of papers by Strange
and coworkers (Strange and Phillips,
1984; Strange et al.,
1982; Strange et al.,
1984) showed that larval Aedes dorsalis exposed to
alkaline media (pH 10.5) high in HCO3– (up to 250
mmol l–1) eliminate this ion via rectal
HCO3–/Cl– exchange. It is not
clear from the available data whether the rectum of larval Aedes
aegypti plays a role in acid–base homeostasis. We have found that
larval A. aegypti has a similar ability to tolerate highly alkaline
media without ill effect, at least in media rendered alkaline using NaOH
(Clark et al., 2004). Under
these conditions, the pH within the rectal lumen of larval A. aegypti
is always acidic in vivo (pH <6.2). The pK of
H2CO3/HCO3– is 6.4 at
25°C (Weast et al., 1986).
Most HCO3– excreted into the rectum at the
observed pH <6.2 would form CO2, assuming equilibrium is reached
by the time the excretory product is eliminated. Any CO2 so formed
would then most likely diffuse through the tissues and out through the
cuticle, resulting in net acid excretion
(Wigglesworth, 1938). If the
physiology of acid–base regulation is similar in larvae of A.
aegypti and A. dorsalis, the high rates of
HCO3– excretion observed in the rectum of A.
dorsalis (Strange and Phillips,
1984; Strange et al.,
1984) may have been induced by the high
HCO3– concentration of the medium (250 mmol
l–1) rather than by its alkaline pH (pH 10.5). This deserves
further study.
The relative contributions of the Malpighian tubules, midgut and hindgut in secretion of the acid observed in the rectal lumen were not determined. We could not measure mitochondrial luminosity of the hindgut due to interference from non-specific fluorescence of lumen contents, which were much more difficult to remove from this region of the alimentary canal. An increase in mitochondrial luminosity would not necessarily indicate a direct role in acid–base transport, however. Elevation of Malpighian tubule secretion rates, observed in acidic media, requires increased rates of rectal recovery of solutes such as K+, Cl–, etc., that drive the formation of Malpighian tubule secretions. Changes in energy demands of the rectum in response to ambient pH would therefore provide little information regarding acid–base transport by this organ.
The role of the AP in acid–base homeostasis
Acid efflux has been shown in the AP of larval Aedes aegypti in
neutral media (Donini and O'Donnell,
2005). In the present study, the changes observed in pH within the
AP in response to changes in ambient pH are not consistent with an active role
of these organs in acid–base homeostasis. Instead, the evidence suggests
that acid–base flux across the AP is passive. First of all, one might
expect the AP to become more alkaline, rather than acidic, if excreting acid,
and to become more acidic if excreting base – in fact, the reverse
occurs. Second, the change in pH within the papillae upon transfer from acidic
to alkaline media is not reversed during at least 24 h of exposure, suggesting
limited ability to regulate flux over this time scale. The passive role of the
AP in acid–base homeostasis is supported by comparison of the phenotypic
plasticity of the AP in response to pH and to NaCl. It is well established
that active NaCl uptake from dilute media occurs in the AP
(Wigglesworth, 1933;
Wigglesworth, 1938;
Koch, 1938). AP of larvae
reared in dilute media show increased size and mitochondrial densities
contributing to greater active NaCl absorption from the medium
(Edwards and Harrison, 1983;
Koch, 1938;
Wigglesworth, 1938). In the
present study, we demonstrated that the size and mitochondrial densities of
the AP are all reduced, rather than increased, in acidic media relative to
those from larvae reared in neutral and alkaline media (in the presence of
NaCl). Reducing the relative surface area of the highly permeable cuticle
appears to be a mechanism to reduce rates of passive transcuticular
H+ influx into the AP. The reduction in mitochondrial densities in
acidic media is also not consistent with an active role of the AP in acid
excretion. The hypothesis that the AP are important sites of active
acid–base excretion in acidic media is therefore not supported.
No evidence was obtained supporting the AP as major sites of active acid–base excretion in alkaline media. Size and mitochondrial densities of the AP are similar in larvae reared in neutral and alkaline media.
The response of the AP to acidic media is influenced by the presence or
absence of NaCl. The AP were reduced in size in acidic media in the presence
of NaCl, but not in its absence. This suggests a trade-off between NaCl uptake
and acid–base homeostasis occurring in the AP of larvae in dilute,
acidic media. In a wide variety of aquatic organisms, death in acidic water is
due primarily to loss of Na+, rather than failure of pH homeostasis
(Vangenechten et al., 1989;
Havas, 1981;
Havas and Advokaat, 1995;
Lin and Randall, 1995). This
appears to be related to Na+/H+ exchange mechanisms
(Stobbart, 1971). In the fish
gill, for example, Na+ uptake is driven by active H+
secretion. Increased ambient H+ concentrations therefore increase
the electrochemical gradients opposing H+ secretion, reducing
Na+ uptake (Lin and Randall,
1995). Similarly, larvae of Aedes aegypti and Culex
quinquefasciatus show decreased Na+ uptake rates during acute
exposure to acidic water (pH 3.5) (Patrick
et al., 2002). It thus appears that AP surface area does not
decrease in dilute media of low pH, because a reduction in size of the AP in
dilute, acidic media would compromise NaCl uptake leading to the failure of
Na+ homeostasis. If such a trade-off exists, A. aegypti
larvae appear to be able to minimize its effects
(Clark et al., 2004).
Intriguingly, the apical surface area of fish gill chloride cells, also
involved in the uptake of ions from dilute media, is reduced during acid
exposure (Goss et al., 1995).
Could reduced surface area of permeable Na+ uptake surfaces, a
response driven by the deleterious consequences of high rates of passive
H+ influx, contribute to the trade-off between Na+ and
H+ homeostasis in a variety of animals exposed to acidic water?
It is highly unlikely that the decrease in size of the AP of larvae reared in acidic media containing NaCl is a response to the increased Cl– concentrations resulting from the HCl added during adjustment of the pH of the rearing medium. The medium [Cl–] was 59.9 mmol l–1, and the small amounts of HCl required to adjust the pH to 4 were of the order of a few millimolar. In addition, the length and mass-specific length of the AP of larvae reared in acidic media in low-NaCl conditions (with pH adjusted using HCl) were not reduced compared with those of larvae reared in deionized water (0 g l–1, see Fig. 2).
During the course of this investigation, we repeated classic studies
documenting the influence of salinity on the size of the AP
(Wigglesworth, 1938;
Koch, 1938), in order to
determine the relative magnitude of the effects of NaCl and pH on AP size.
Those studies had found that the AP of larval mosquitoes reared in dilute
media were larger than those of larvae reared at higher salinities, although
AP of Aedes aegypti did not respond as strongly to ambient salinity
as did those of several other species. As reported in those studies, we too
found that AP are longest in larvae reared in dilute media. However, when
scaled for mass, we did not observe any relationship between salinity and AP
length. Under the conditions of this study, the effects of salinity on the
length of the AP appear to be more strongly associated with allometric effects
of salinity on overall growth, rather than changes in the relative sizes of
ion uptake surfaces. We do not question the role of the AP in NaCl uptake.
Note, however, that pH (in the presence of NaCl) has a much greater effect on
AP size than does salinity in this species suggesting that acid–base
flux into the AP in acidic media is of considerable physiological
significance. It is possible that estimation of total surface area or a
greater effort to eliminate NaCl (for example by feeding larvae NaCl-free
food) may have resulted in a stronger relationship between mass-specific
length and salinity in the present study.
Physiology of acid–base regulation in acidic media
In acidic media, larvae greatly increase drinking rates. This increase is
likely to impose a considerable energy cost on the animal. The insect
excretory system drives water movement by solute transport. Larvae in acidic
media ingest much greater fluid volumes, the ingested fluid contributes to the
acid load to be eliminated, and ions used to drive urine secretion must be
recovered from the excreta prior to its elimination. Why then would larvae
increase drinking rates in acidic media? Two hypotheses come to mind.
According to one hypothesis, larvae exposed to acidic media increase drinking
rates in order to reduce the transepithelial H+ gradient opposing
clearance of H+. This would resemble the mammalian kidney, which
can only excrete H+ into filtrate of pH >4.5 but can increase
clearance of H+ by addition of buffers and NH3 to the
urine. We hypothesize that an increased volume of fluid of a given pH and
buffer capacity allows a greater acid load to be cleared without increasing
the driving force opposing H+ excretion. For this to work, the
increase in clearance capacity must compensate for the additional acid load
ingested with the medium. A similar hypothesis was proposed to explain an
increase in drinking rates observed in larvae exposed to elevated salinity
(Clements, 2000).
A second hypothesis that might explain the increase in drinking rates in acid water is based on Na+/H+ exchange processes (discussed above). It is thus conceivable that the increase in drinking rates in acidic media functions to increase Na+ ingestion, offsetting the reduction in Na+ influx caused by elevated ambient H+ concentrations. This hypothesis must be rejected in the present study, however. Larvae ingested the medium at similar rates in acidic media differing in NaCl concentration. Indeed, drinking rates increased approximately 5-fold between pH 4 and pH 7 in low-NaCl RS, but only by 2- to 3-fold in RS containing NaCl (59.9 mmol l–1).
Physiology of acid–base regulation in alkaline media
We had expected to find that larvae exposed to alkaline media would excrete
fluid more alkaline than the hemolymph, although not necessarily more alkaline
than the environment, to remain in pH balance. We were surprised to find that
the excretory system of larvae acclimated to highly alkaline media (pH 11)
actually excreted fluid more acidic than the hemolymph. Animal metabolism
always produces acids, due to the generation of CO2 and/or lactic
acid during metabolism. Additional acids are formed during processes such as
triglyceride or protein catabolism. Depending on an animal's physiological
state, however, excreted fluids may be either acidic or alkaline. Data
presented by Stobbart (Stobbart,
1971; Stobbart,
1974) show that larval Aedes aegypti may either alkalize
or acidify the surrounding medium, depending on their state of ionic
homeostasis and the ionic composition of the medium. Vanatta and Frazier
(Vanatta and Frazier, 1981)
found that frogs rendered alkalotic by NaHCO3–
injection excreted base via transepithelial processes. Excretion of
HCO3– would allow larval mosquitoes in highly
alkaline media to excrete fluid that is more alkaline than the hemolymph yet
more acidic than the environment. Because the pK of the transition
from HCO3– to CO32– is
pH 10.25 at 25°C (Weast et al.,
1986), HCO3– would act as an acid in
media above this pH value. It is therefore not unexpected that the larvae show
net acid excretion in highly alkaline media.
There are two ways in which larvae can excrete fluid more acidic than the hemolymph during steady-state exposure to alkaline media: (1) the larvae may neutralize ingested base-utilizing acids produced during metabolism, or (2) the larvae may excrete net base (or absorb acid) through the actions of extrarenal organs. If active excretion of base (either by the excretory system or by extrarenal organs) increases with ambient pH, then the energy demands of the organs involved are expected to increase as the rate of transport and the opposing concentration gradients increase. Larvae reared in high ambient pH did not possess elevated mitochondrial densities in any renal or extrarenal organ, and the AP were not increased in size in response to alkaline media. We have also found that the metabolic rates of larvae exposed to pH 11 media are the lowest observed under any conditions of pH or salinity (J. M. McLister and T.M.C., unpublished observation). Larvae thus appear to possess the remarkable ability to remain in pH balance in highly alkaline water without excreting base or, equivalently, absorbing acid. They appear to depend instead on metabolic acid production to neutralize ingested base. If so, the relatively low drinking rates observed in alkaline water may allow the larvae to remain in pH homeostasis by reducing the amount of base to be neutralized. To the best of our knowledge, this strategy, in which pH homeostasis is maintained in highly alkaline media by excreting fluid more acidic than the hemolymph, has not been reported in any other animal. Few studies have addressed the physiology of acid–base homeostasis in alkaline media, however, and it is quite likely that this ability is not unique to the larval mosquito.
Larval Aedes aegypti develops well in highly alkaline media. Larvae of this species live in small containers of water, generally containing some plant materials. Such habitats are not highly alkaline. It is possible that the ability to survive under these conditions is an adaptation inherited from an ancestral species that is not currently useful. However, if this ability imposed a significant cost it is likely that it would have been lost. It therefore seems likely that the ability of larvae Aedes aegypti to survive in such media is a fortuitous consequence of physiological characteristics, such as low cuticular permeability, air breathing, and the generation of a highly alkaline midgut lumen, that evolved in other contexts.
We have earlier reported that high pH reduces growth rates, and increases
developmental times, of larval Aedes aegypti
(Clark et al., 2004). We have
found in the present study that larvae acidify alkaline media. Larval
mosquitoes inhabiting small volumes of alkaline water may thus make their
surroundings more suitable for their own growth and development, and
presumably also the survival of the organisms upon which they feed. Early
instars appear to be more susceptible to extreme pH than later ones (T.M.C.,
unpublished observations). Neutralization of highly alkaline media by larval
metabolic processes could therefore enhance the suitability of small volumes
of water for future generations.
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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. (B) Effects of ambient pH on percentage body water. Body
water was reduced in larvae chronically exposed to acidic media, and was
elevated when larvae were acutely exposed to more acidic media (single factor
ANOVA of arcsine-transformed body water ratio). The presence or absence of
NaCl did not influence the effects of acute pH challenges on body water. RS 7
represents larvae reared and assayed in RS 7, RS 7–3 represents larvae
reared in RS 7 and assayed in RS 3, RS 4 represents larvae reared and assayed
in RS 4, and RS 4–3 represents larvae reared in RS 4 and transferred to
RS 3. For larvae reared and assayed in low NaCl conditions, low-NaCl RS 7
represents larvae reared and assayed in low-NaCl RS 7, while low-NaCl RS
7–3 represents larvae reared in low-NaCl RS 7 and assayed in low-NaCl RS
3. Data are presented as means ± s.e.m.
