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Department of Biology, University of Central Arkansas, Conway, Arkansas 72035-0001
In Aplysia intestine,
stimulation of Na+ absorption with
luminal alanine increases apical membrane
K+ conductance
(GK,a), which
presumably regulates enterocyte volume during stimulated
Na+ absorption. However, the
mechanism responsible for the sustained increase in plasma membrane
K+ conductance is not known for
any nutrient-absorbing epithelium. In the present study, we have begun
to test the hypothesis that the alanine-induced increase in
GK,a in
Aplysia enterocytes results from
exocytic insertion of K+ channels
into the apical membrane. We used the fluid-phase marker horseradish
peroxidase to assess the effect of alanine on apical membrane
exocytosis and conventional microelectrode techniques to assess the
effect of alanine on fractional capacitance of the apical membrane
(fCa). Luminal
alanine significantly increased apical membrane exocytosis from 1.04 ± 0.30 to 1.39 ± 0.38 ng · min
1 · cm
2.
To measure fCa,
we modeled the Aplysia enterocyte as a
double resistance-capacitance (RC) electric circuit arranged in series. Several criteria were tested to confirm application of the model to the
enterocytes, and all satisfied the model. When added to the luminal
surface, alanine significantly increased
fCa from 0.27 ± 0.02 to 0.33 ± 0.04 (n = 10)
after 4 min. There are two possible explanations for our findings:
1) the increase in exocytosis, which
adds membrane to the apical plasma membrane, prevents plasma membrane
fracture, and 2) the increase in
exocytosis delivers K+ channels to
the apical membrane by exocytic insertion. After the alanine-induced
depolarization of apical membrane potential (Va), there is
a strong correlation (r = 0.96)
between repolarization of
Va, which
reflects the increase in
GK,a, and
increase in fCa. This correlation supports the exocytic insertion hypothesis for activation of
GK,a.
membrane capacitance; potassium channels; nutrient absorption; sea hare
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