Volumetric and ionic responses of goldfish hepatocytes to anisotonic exposure and energetic limitation
M. V. Espelt1,
P. N. Mut1,
G. Amodeo2,
G. Krumschnabel3 and
P. J. Schwarzbaum1,*
1 Instituto de Química y Fisicoquímica Biológicas
(Facultad de Farmacia y Bioquímica), Universidad de Buenos Aires,
C1113AAD Buenos Aires, Argentina
2 Laboratorio de Biomembranas (Facultad de Medicina), Universidad de Buenos
Aires, C1121ABG Buenos Aires, Argentina
3 Institut für Zoologie, Abteilung für Ökophysiologie,
Universität Innsbruck, A-6020, Austria

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Fig. 2. Time course of volume changes in hepatocytes from goldfish, trout and rat,
assessed by quantitative phase-contrast microscopy. (A) Total volume
(V) changes of hepatocytes from goldfish exposed to 180 mosmol
l-1 medium at pH 7.45. Hepatocytes were isolated in
collagenase-containing medium (filled circles) or in collagenase-free medium
(open circles). (B) Relative volume (Vr) changes of
hepatocytes of rat (triangles) and trout (squares) exposed to 180 mosmol
l-1 medium at pH 7.45 and of goldfish hepatocytes (circles) exposed
to 180 mosmol l-1 at pH 7.8. Values are means ± S.E.M.
(N=4). Lines represent the empirical fit to data, with values of the
parameters given in Table 1 and
in the Results section.
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Fig. 1. Time course of total volume (V) change in goldfish hepatocytes,
assessed by quantitative phase-contrast microscopy. Cells were exposed to
media of the various osmolarities indicated at pH 7.45 and to L-alanine,
aminooxyacetic acid (ALA-AOA). Results are means ± S.E.M.
(N=4; in certain points, the error bars lie within the symbol). Lines
represent the exponential fit to experimental data with parameters of best fit
given in Table 1. The inset
shows phase-contrast micrographs of goldfish hepatocytes in 300 mosmol
l-1 (top panels) and 120 mosmol l-1 media (bottom
panels).
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Fig. 3. Relative volume (Vr) versus time in goldfish
hepatocytes incubated in control medium A or in medium with (A) iodoacetic
acid (IAA) or (B) cyanide plus iodoacetic acid (CN-+IAA).
Calibration was performed with anisosmotic media of 264 mosmol l-1
(medium H) and 308 mosmol l-1 (medium J). Results are means
± S.E.M. (N=4).
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Fig. 4. Relative volume (Vr) versus time in
hepatocytes from (A) goldfish and (B) rat incubated in control media (denoted
as A for goldfish cells and C for rat cells) or in medium with cyanide
(CN-). Calibration was performed with anisosmotic media as follows:
(A) 264 mosmol l-1 (medium H) and 308 mosmol l-1 (medium
J); (B) 225 mosmol l-1 (medium H) and 293 mosmol l-1
(medium J). Results are means ± S.E.M. (N=4).
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Fig. 5. Rates of 86Rb+ influx in goldfish hepatocytes during
44 min of exposure to control medium (A), 180 mosmol l-1 medium
(HY), isosmotic media with cyanide (CN-), iodoacetic acid (IAA) and
cyanide plus iodoacetic acid (CN-+IAA). Fluxes were measured at 4
min, 14 min, 24 min and 44 min after the start of the experiment. Results are
means + S.E.M. (N=4). An asterisk indicates P<0.05 with
respect to isosmotic control values.
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Fig. 6. Rates of 86Rb+ efflux in goldfish hepatocytes during
44 min of exposure to control medium (A), 180 mosmol l-1 medium
(HY), isosmotic media with cyanide (CN-), iodoacetic acid (IAA),
and cyanide plus iodoacetic acid (CN-+IAA). Fluxes were measured at
4 min, 14 min, 24 min and 44 min after the start of the experiment. Results
are means + S.E.M. (N=4).
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Fig. 7. Rates of 86Rb+ efflux in goldfish hepatocytes exposed
to 180 mosmol l-1 medium and pH 7.45, pH 7.8 or pH 7.45 +
N-ethylmaleimide (NEM). Results are means + S.E.M. (N=4). An
asterisk indicates P<0.05 with respect to isosmotic values.
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Fig. 8. Intracellular Na+ (nmol 10-6 cells-1)
versus time in hepatocytes of goldfish exposed to control medium (A),
cyanide (CN-), ouabain (OB) and isotonic 100 mmol l-1
MgCl2 (Na+-free medium). Results are means ±
S.E.M. (N=4).
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© The Company of Biologists Ltd 2003