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Calcium-activated potassium channels in chondrocytes
BIOCHEMICAL
Vol. 182, No. 3, 1992
AND BIOPHYSICAL RESEARCH COMMUNICATIONS Pages 1429-1434
February 14, 1992
CALCIUM-ACTIVATED
POTASSIUM
CHANNELS
IN
CHONDROCYTES M.Grandolfo*, *Din
P. D’Andrea*.
Biochimica, OIst.
Received
di
M. Martina*,
Biofisica
e Chimica
Fisiologia,
December
Via
29,
F. Ruzzier’,
delle
A.Fleming Trieste,
and
Macromolecole,
22, Universitl Italy
F. Vittur*
Via di
A.Valerio
Trieste,
22,
34127
1991
The presence of calcium-activated potassium channels in chondrocytes of growResults obtained with furaon cultured resting ing cartilage was tested. chondrocytes indicate that he cells respond to an elevation of extracellular calcium concentration ( [Ca t+ 1 1 f om 0.1 to 2 mM increasing the intracellu1 f rom 117 to 187 nM. This lar concentration of the ion Y [Cah+I. increment may be blocked by 3pM La3+. P tch clan& experiments in cell-attached configuration showed that, when [Ca 1+ Ii rises, the open probability (PO) of the K+ channels increases. Increments in both PO and channels can be obtained after applying 2.5pM A23187 with 2mM the results demonstrate that, in chondrocytes,a channels is present and their activity is related to an B 1992
The
Academic
Press,
membrane
cytes
Inc.
potential
of growth
plate
approaching
the
tion
membrane
of the
other
pump,
the
tive
types
K+ channels.
channels
that
are
frequently
Ca2+ -activated free
voltage
was
sensitive
modulated Kt-channels
Ca2+ concentration
it
that
system
(3)
by calcium in and the
chondrocytes. K+-channel
a key
least
in
interest
the
regula-
to study
(>
200
activity
kinds
and the that pS) Since
aim of this The
include
three
demonstrated
the
chondro-
differentiation
role
systems
activated
and TEA.
(21,
cell
in
correlation
the
Na*-Kt
of
conduc-
volume
sensitive
chondrocytes
from
voltage
dependent
channels
of this
work
was to between
K+ kind
look
for
cytosolic
was investigated. 0006-291x/92
1429
the
membrane.
and at
conductance
to quinidine
of
of
these
the Ca2*
activity
stage
therefore
plasma
et al.
high
the
Kt plays
is
found
sated,
Grandolfo have
are
(1).
and
it
potassium
with
of chondrocyte
(2)
Recently
cartilage
surface
co-transport
the
resting
change
potential
Nat-K+-2Cl-
channels:
intracellular
cartilage
systems
cell
the
mineralizing
K+ transporting In
and
$1.50
Copyright 0 1992 by Academic Press, Inc. All righfs of reproduction in any form reserved.
Vol.
182,
No.
Lsolation
3, 1992
md
BIOCHEMICAL
culture
ti
AND
PreoS8eOUg
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
chondrocvtes
Scapulas from 40 to 70 kg pigs were excised from animals imnediately after death. The scapulas were freed of perichondrium and the cartilagineous portion was cleaved off. The resting region, furthest from the mineralizing surface, was selected and dissected as already described (4). The enzymatic disaggregation of the tissue and the chondrocyte plating and culture conditions have been previously reported (5). Furameasurements & jCa’+li These measurements were carried out as described by D’Andrea et al. (5). Briefly, 48 hrs serum starved confluent cultures were treated by trypsin (0.05X)-EDTA (0.02%) solution. The cell suspension in DMEM was incubated with 5 pM fura-2-acetoxy methylester (Molecular Probes, USA) for 1 h at 37’C. The cells where then rinsed with buffer (in mM: 140 NaCl, 5 KCl. 1.5 M&12, 5 glucose, 10 Hepes (Sigma), 0.1% bovine serum albumin, fraction V (Sigma); pH 7.4 with Tris), and resuspended at a concentration of IO6 cells/ml. When neces ary, cells where washed twice in the above buffer solution to which 0.1 IIS! CaS+ was added. To obtain 2 r&l or higher calcium concentrations, a few microliters of stock CaCl2 solution were added. Fluorescence was measured under continuous stirring in a Jasco spectrofluorometer. Signal calibration was performed as described by Meldolesi et al. (6). Patch-clrecordinConfluent cells were employed for the electrophysiological experiments which were performed as described by Grandolfo et al. (3). The cells were rinsed and then maintained for 1 h in the following solution (in mM): 130 NaCl, 3 KCl, 0.1 CaC12, 10 Na-Hepes: pH 7.2. Pipettes were filled with the same solution as above. Single channel currents were recorded in the cell-attached and the outward current, i.e. current flowing from the cytoconfiguration, plasmic to the external side of the membrane, are shown as positive deflections. The electrophysiological experiments were done at room temperature (20-25 ‘C), whereas the fluorescence was measured at 37 OC.
RESULTS To evaluate maintained
the in
by using
role
of
bathing
solutions
fluorescence
Fura-
records
Fig.
[Ca’+li
in response
to
logical
saline of
at
low
content
Ca 2+ concent
resting
[Ca2+Io.
The cells,
further
( widely (Pig. in
1 B). the
. The
used Ca 2* channel Moreover, fluorescence
when
entry blockers
the
signal
were
studied
regulate
their
is
of not
cells
are
are
observed
1430
from [Ca2+Io
blocked
) but
is
in
mM) respond
[Ca”Ii
increments
Ca2+
rat ion
maintained
= 0.1
[Ca2+lo up to 1.8 - 2mM, by increasing
[Ca’+li
chondrocytes
chondrocytes
([Ca2+Io
Additional
K+-channels,
of
methods.
that
calcium
alter
no changes
different
of
not
La3+
of
Change83
to 187 f 23 nM (n = 37).
3vM
the
1 A show
20)
verapamil
activity
on
and electrophysiological
in
crease
ICa’+Ii
(data
to
an
in-
117 f 17 nM (n = up to 15 a&l does by nifedipine
completely
depolarized
a physio-
by not
inhibited
and by
KC1 (40 mM), shown).
These
Vol. 182, No. 3, 1992
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
200 z c
100 I
.-
1.8mM
[Ca2’lo
200
7
N
%iI
100 I
Pig. 1 Influence
of tCa**l on ICa**l. and blockage A) The cells we eOloaded witch fur-a-z, and [Ca*+l The [Ca I+ 1 was then raised to the was esffmated from the fluorescence ion (B) The cells maintained at O.ldl [Ca calcium entry was observed when
findings
suggest
at
Ca 24 channels
dependent The activity studied
that,
of
using
ty occurs
A 0.1
is
(Pig.
mM
are
K+ channels the
When [Ca2+lo
least
patch
raised 2A).
under
our
of
calcium
entry
by
La3’.
initially exposed (A) to O.lmM indicated values and the [Ca2’li (see Materials and methods). were treated by 3 pM La3*: no
experimental
conditions,
voltage-
undetectable. in
resting
clamp from
B
I
--
technique
0.1
Likewise,
chondrocytes
to 2mM,
in
tCa2+lo,
different
cell-attached
increment
an
at higher
the
at
open
was
configuration.
of the the
[Ca2*lo
K* channel
activi-
probability,
PO, as
B
[Ca2*],
2 mM[Ca2+lo
10pA Vpipz
Vpip
-3OmV 20
hnV)
msec
pis.s
Single cytes.
channel
currents
across
voltage-activated
K*
channels
in
chondro-
(A) Representative currents recorded in cell-attached configuration at a -3OmV pipette pqt+ential (Vpip) when exposing the cell to 0.1 mM (upper trace) or 2mM tCa lo (lower trace). (B) Voltage dependence of channel activity expressed as open probability (PO) at (0-e) O.lmM or (A-A) 21d4 tCa2+lo. 1431
Vol.
182, No. 3, 1992
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
600,
[Ca2fo=
2 ti~M
A
400,
[Ca2+]
i
nM
d+
200,
A23187
1 min.
I
a
u Cytosolic treated
with
[Ca 2+ 1 chanses A23187.
and
single-channel
K+
currents
in
chondrocytes
Chondrocytes were exposed to 2mM [Ca2’Io and A23187 wa added to a concentration of 2.5nM (see arrow). (A) A typical trace of [Ca82+Ii variation by furaafter ionophore addition and as a function of time, and determined (Bl Single-channel K+ currents measured at a Vpip of -40mV at the basal (a), transient fbl and final steady-state (cl levels of [Ca”It.
a function resting
of
Vpip
membrane
mM [Ca2+lo
(pipette
potential
(Po=O)
when
extracellular of the
increase
of
reached
the
K+ channels creased an increase
of
A23187
terms
3 8).
In
the
unitary
in
the
presence
600 nM (Fig.
3 AI.
fact,
PO and
unitary
at Vpip=O current
of
pS,
of
of about
1432
in the
15%. The
the
at
0.1
at
0.1
2 mM
or
respectively).
2 mM [Ca2*lo, 350
from
At
mean slope
of
nM,
amplitude
the PO changes
observed
presence
n=4.
2B).
observed
As a consequence, current
about
is
observed
in the
112*17
a plateau
of
are
and
180 nM to
is
activity
incubated
n=4,
(Figure
activity
evident
are
pS,
from
of almost
( in (Pip.
but
differences
chondrocytes (96?35
increases
= 0) no channel
a modest
ionophore
[Ca2+li
a peak
voltage)
No significant
Ca 2*
addition
(Vpip
while
[Ca*+ IO (Po=O.OOlI. conductance
applied
The
induces after
an
having
the
activity
1 is
highly
in-
to 0.02
with
is
evi-
0.001
phenomenon
2 mM
more
of
Vol.
182, No. 3, 1992
dent
BIOCHEMICAL
at a Vpip=-4OmV
current
increases
when the
AND BIOPHYSICAL
PO changes
from
RESEARCH COMMUNICATIONS
0.85
to
0.3
and
the
unitary
of 80%.
QISCUSSION The
aim of
channel
experiments
activity.
amount Ca2+
our
Two facts
of extracellular Kt
The
variation
physiological of Ca ”
zation
from
[Ca*+ Ii
the
um channels of
is
in
experimental
the
rise,
cells
rapidly
of K+- channels allows
and
(see
Fig.
were
obtained
fura-
in
iB1,
depletion
lar
space.
and the
to
as
already
when
using
shows of
A clear
different
that
clamp
time
are
[Ca’+Ii
for
other
ionophore
A23187
evokes
stores was observed levels
instead
(see
of
a marked and to
between Fig. 1433
2B).
not
presence
of
(8.9)
or
influx
the
activity
cells,
of
these
of
Similar
of from of
chan-
the
level
the
may
activity
which
the
changing
the
observed
on the
for
and
a [Ca2+lo
the
(11-131.
transient
voltage cells
excitable
to
types
blocker
were
conductance
of calci-
active”
channels”
cell
of the
following
effect
related
within
through
these
“tonically
The
strictly
in
in
of
elevation
are
However,
has a significant
recordings.
[Ca2+Io
changes
found
of
changes
( an aspecific
of Ca 2+,
as “maxi-K+
shown an
(10)
the
a class
sustained
ICa’+Ii
the
that
of Ca*+ mobili-
channels
verapamil.
K*-
as a consequence
detectable
The entry
example
[Ca’+ Ii
intracellular link
no
channels”
in
patch
open
fact,
and
be classified
the
response
the
our
them
probability
“fast rise
not
of
seems to occur
calcium
is
by KCl.
as for
by
but
entry
channel
by nifedipine
modulated
as a result
a little
these
In
that
by 3pM La3+
Apparently,
inactivating
and not
Only
second,
only
on the
first,
increase
occur
inhibited
depolarized
The
to
space
of
are an
[Ca’+Ii
results:
and,
and
The calcium
of Ca 2+ -channels,
be hypothesized.
nels
(7).
type
blocked
[Ca’+Ii
appears
of
present
following
conditions.
were
was not
some types the
as this
by the
stores.
(7)).
(WCs)
these
[Ca’+Iit
completely
channels
an influence
present
extracellular
observed
operated
when
of
the
as it
calcium
are
intracellular
has been
proved
(O.l-2mM).
from
prove
modifies
channels
limits
entry
are
calcium
activated
ICaZ+lis
was to
open
[Ca’+Ii results
[Ca2+Io.
[Ca2+Ii, the the
The due to
extracelluK+channels
Vol.
182,
All
No.
these in
channels is
are
It
growth
is
the
clearly
present
that
(14).
Although
&Q
membrane
and tissue
not
only
(D.l-2mM),
potential
that
total
these
calcium
as a function these
situation,
cart i lage , may influence cyte
BIOPHYSICAL
RESEARCH
that but
the
also
COMMUNICATIONS
lCa’*li
that
depends
CaZt-activated
on Kt
in chondrocytes.
varies
b
range
to hypothesize known
AND
demonstrate
physiological
plate,
surface to
the
tempting
tion.
BIOCHEMICAL
results
[Ca2+lo
It
3, 1992
the the
(11,
the
on cell
in
from
can only
existing
conductances
with
in calcifica-
different the
in part
gradient,
differentiation,
a role the
distance
studies
calcium membrane
may play
concentration, of
in vitro
changes
zones
mineralization be extrapolated
Jo w an
matrix
of
effect vesicle
in on
growth chondro-
formation
calcification.
ACKNOWLEDGMENTS This work Miss M.T. Fondo per ter, and scapulas.
was supported by research grants from CNR and MURST, Italy. We thank Nicodemo for her valid technical assistance. We also acknowledge the lo Studio delle Malattie de1 Fegato for use of the spectrofluoromethe Uanetto Delicatessen Factory for the generous supply of pip
REFERENCES 1.
2. 3. 4. 5. 6. 7. a. 9. ::: 12. 13. 14.
Edelman. A., Thil, C.L., Garabedian, M., Plachot, J.J., Guillozo, H., Fritsch, J., Thomas, S.R., Balsan, S. (1985) Min. Electr. Metab. 11,97-105. Grinstein, S. and Dixon, S.J. (1989) Physiol. Rev. 69.417-481. Crandolfo, M.. Martina, M., Ruzzier, F., Vittur, F. (1990). Calcif. Tissue Tnt. 47, 302-307. Vittur, F., Pugliarello, M.C., de Bernard, B. (1971) Experientia 27,126-127. D’Andrea, P., Grandolfo, M.. de Bernard, 6. Vittur, F. (1990) Exp. Cell Res. 191, 22-26. Meldolesi I J., Huttner, W.B., Tsien, R.Y., Pozzan, T. (1984) Proc . Nat. Acad. Sci. USA 81,620-624. Nemeth, E.F. (1990) Cell Calcium 11.323-327. Benham, C.D. and Tsien, R.W. (1987) in Cell calcium and the control of membrane transport (L. J. Mandel, D.C. Eaton, Eds), pp 45-64. The Rockefeller University Press, New York. Rosenberg, R.L., Hess, P., Tsien. R.W. (1988) J. Gen. Physiol. 92.27-54. Meldolesi, J. and Pozzan, T. (1987) Exp. Cell Res. 171, 271-283. Latorre, R.. Vergara M.C., Hidalso, C. (1982) Proc. Natl. Acad.Sci. USA 79.805-809. Schwarz, W.and Passow, H. (1983) Ann. Rev. Physiol. 45.359-374. Latorre. R., Oberhauser, A.. Labarca, P.. Alvarez, 0. (1989) Ann. Rev. Physiol. 51.385-399. Howell, D.S., Delchamps, E., Riemer. W., Kiem, I. (1960) J. Clin. Invest. 39.919-929. 1434
Vol. 182, No. 3, 1992
AND BIOPHYSICAL RESEARCH COMMUNICATIONS Pages 1429-1434
February 14, 1992
CALCIUM-ACTIVATED
POTASSIUM
CHANNELS
IN
CHONDROCYTES M.Grandolfo*, *Din
P. D’Andrea*.
Biochimica, OIst.
Received
di
M. Martina*,
Biofisica
e Chimica
Fisiologia,
December
Via
29,
F. Ruzzier’,
delle
A.Fleming Trieste,
and
Macromolecole,
22, Universitl Italy
F. Vittur*
Via di
A.Valerio
Trieste,
22,
34127
1991
The presence of calcium-activated potassium channels in chondrocytes of growResults obtained with furaon cultured resting ing cartilage was tested. chondrocytes indicate that he cells respond to an elevation of extracellular calcium concentration ( [Ca t+ 1 1 f om 0.1 to 2 mM increasing the intracellu1 f rom 117 to 187 nM. This lar concentration of the ion Y [Cah+I. increment may be blocked by 3pM La3+. P tch clan& experiments in cell-attached configuration showed that, when [Ca 1+ Ii rises, the open probability (PO) of the K+ channels increases. Increments in both PO and channels can be obtained after applying 2.5pM A23187 with 2mM the results demonstrate that, in chondrocytes,a channels is present and their activity is related to an B 1992
The
Academic
Press,
membrane
cytes
Inc.
potential
of growth
plate
approaching
the
tion
membrane
of the
other
pump,
the
tive
types
K+ channels.
channels
that
are
frequently
Ca2+ -activated free
voltage
was
sensitive
modulated Kt-channels
Ca2+ concentration
it
that
system
(3)
by calcium in and the
chondrocytes. K+-channel
a key
least
in
interest
the
regula-
to study
(>
200
activity
kinds
and the that pS) Since
aim of this The
include
three
demonstrated
the
chondro-
differentiation
role
systems
activated
and TEA.
(21,
cell
in
correlation
the
Na*-Kt
of
conduc-
volume
sensitive
chondrocytes
from
voltage
dependent
channels
of this
work
was to between
K+ kind
look
for
cytosolic
was investigated. 0006-291x/92
1429
the
membrane.
and at
conductance
to quinidine
of
of
these
the Ca2*
activity
stage
therefore
plasma
et al.
high
the
Kt plays
is
found
sated,
Grandolfo have
are
(1).
and
it
potassium
with
of chondrocyte
(2)
Recently
cartilage
surface
co-transport
the
resting
change
potential
Nat-K+-2Cl-
channels:
intracellular
cartilage
systems
cell
the
mineralizing
K+ transporting In
and
$1.50
Copyright 0 1992 by Academic Press, Inc. All righfs of reproduction in any form reserved.
Vol.
182,
No.
Lsolation
3, 1992
md
BIOCHEMICAL
culture
ti
AND
PreoS8eOUg
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
chondrocvtes
Scapulas from 40 to 70 kg pigs were excised from animals imnediately after death. The scapulas were freed of perichondrium and the cartilagineous portion was cleaved off. The resting region, furthest from the mineralizing surface, was selected and dissected as already described (4). The enzymatic disaggregation of the tissue and the chondrocyte plating and culture conditions have been previously reported (5). Furameasurements & jCa’+li These measurements were carried out as described by D’Andrea et al. (5). Briefly, 48 hrs serum starved confluent cultures were treated by trypsin (0.05X)-EDTA (0.02%) solution. The cell suspension in DMEM was incubated with 5 pM fura-2-acetoxy methylester (Molecular Probes, USA) for 1 h at 37’C. The cells where then rinsed with buffer (in mM: 140 NaCl, 5 KCl. 1.5 M&12, 5 glucose, 10 Hepes (Sigma), 0.1% bovine serum albumin, fraction V (Sigma); pH 7.4 with Tris), and resuspended at a concentration of IO6 cells/ml. When neces ary, cells where washed twice in the above buffer solution to which 0.1 IIS! CaS+ was added. To obtain 2 r&l or higher calcium concentrations, a few microliters of stock CaCl2 solution were added. Fluorescence was measured under continuous stirring in a Jasco spectrofluorometer. Signal calibration was performed as described by Meldolesi et al. (6). Patch-clrecordinConfluent cells were employed for the electrophysiological experiments which were performed as described by Grandolfo et al. (3). The cells were rinsed and then maintained for 1 h in the following solution (in mM): 130 NaCl, 3 KCl, 0.1 CaC12, 10 Na-Hepes: pH 7.2. Pipettes were filled with the same solution as above. Single channel currents were recorded in the cell-attached and the outward current, i.e. current flowing from the cytoconfiguration, plasmic to the external side of the membrane, are shown as positive deflections. The electrophysiological experiments were done at room temperature (20-25 ‘C), whereas the fluorescence was measured at 37 OC.
RESULTS To evaluate maintained
the in
by using
role
of
bathing
solutions
fluorescence
Fura-
records
Fig.
[Ca’+li
in response
to
logical
saline of
at
low
content
Ca 2+ concent
resting
[Ca2+Io.
The cells,
further
( widely (Pig. in
1 B). the
. The
used Ca 2* channel Moreover, fluorescence
when
entry blockers
the
signal
were
studied
regulate
their
is
of not
cells
are
are
observed
1430
from [Ca2+Io
blocked
) but
is
in
mM) respond
[Ca”Ii
increments
Ca2+
rat ion
maintained
= 0.1
[Ca2+lo up to 1.8 - 2mM, by increasing
[Ca’+li
chondrocytes
chondrocytes
([Ca2+Io
Additional
K+-channels,
of
methods.
that
calcium
alter
no changes
different
of
not
La3+
of
Change83
to 187 f 23 nM (n = 37).
3vM
the
1 A show
20)
verapamil
activity
on
and electrophysiological
in
crease
ICa’+Ii
(data
to
an
in-
117 f 17 nM (n = up to 15 a&l does by nifedipine
completely
depolarized
a physio-
by not
inhibited
and by
KC1 (40 mM), shown).
These
Vol. 182, No. 3, 1992
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
200 z c
100 I
.-
1.8mM
[Ca2’lo
200
7
N
%iI
100 I
Pig. 1 Influence
of tCa**l on ICa**l. and blockage A) The cells we eOloaded witch fur-a-z, and [Ca*+l The [Ca I+ 1 was then raised to the was esffmated from the fluorescence ion (B) The cells maintained at O.ldl [Ca calcium entry was observed when
findings
suggest
at
Ca 24 channels
dependent The activity studied
that,
of
using
ty occurs
A 0.1
is
(Pig.
mM
are
K+ channels the
When [Ca2+lo
least
patch
raised 2A).
under
our
of
calcium
entry
by
La3’.
initially exposed (A) to O.lmM indicated values and the [Ca2’li (see Materials and methods). were treated by 3 pM La3*: no
experimental
conditions,
voltage-
undetectable. in
resting
clamp from
B
I
--
technique
0.1
Likewise,
chondrocytes
to 2mM,
in
tCa2+lo,
different
cell-attached
increment
an
at higher
the
at
open
was
configuration.
of the the
[Ca2*lo
K* channel
activi-
probability,
PO, as
B
[Ca2*],
2 mM[Ca2+lo
10pA Vpipz
Vpip
-3OmV 20
hnV)
msec
pis.s
Single cytes.
channel
currents
across
voltage-activated
K*
channels
in
chondro-
(A) Representative currents recorded in cell-attached configuration at a -3OmV pipette pqt+ential (Vpip) when exposing the cell to 0.1 mM (upper trace) or 2mM tCa lo (lower trace). (B) Voltage dependence of channel activity expressed as open probability (PO) at (0-e) O.lmM or (A-A) 21d4 tCa2+lo. 1431
Vol.
182, No. 3, 1992
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
600,
[Ca2fo=
2 ti~M
A
400,
[Ca2+]
i
nM
d+
200,
A23187
1 min.
I
a
u Cytosolic treated
with
[Ca 2+ 1 chanses A23187.
and
single-channel
K+
currents
in
chondrocytes
Chondrocytes were exposed to 2mM [Ca2’Io and A23187 wa added to a concentration of 2.5nM (see arrow). (A) A typical trace of [Ca82+Ii variation by furaafter ionophore addition and as a function of time, and determined (Bl Single-channel K+ currents measured at a Vpip of -40mV at the basal (a), transient fbl and final steady-state (cl levels of [Ca”It.
a function resting
of
Vpip
membrane
mM [Ca2+lo
(pipette
potential
(Po=O)
when
extracellular of the
increase
of
reached
the
K+ channels creased an increase
of
A23187
terms
3 8).
In
the
unitary
in
the
presence
600 nM (Fig.
3 AI.
fact,
PO and
unitary
at Vpip=O current
of
pS,
of
of about
1432
in the
15%. The
the
at
0.1
at
0.1
2 mM
or
respectively).
2 mM [Ca2*lo, 350
from
At
mean slope
of
nM,
amplitude
the PO changes
observed
presence
n=4.
2B).
observed
As a consequence, current
about
is
observed
in the
112*17
a plateau
of
are
and
180 nM to
is
activity
incubated
n=4,
(Figure
activity
evident
are
pS,
from
of almost
( in (Pip.
but
differences
chondrocytes (96?35
increases
= 0) no channel
a modest
ionophore
[Ca2+li
a peak
voltage)
No significant
Ca 2*
addition
(Vpip
while
[Ca*+ IO (Po=O.OOlI. conductance
applied
The
induces after
an
having
the
activity
1 is
highly
in-
to 0.02
with
is
evi-
0.001
phenomenon
2 mM
more
of
Vol.
182, No. 3, 1992
dent
BIOCHEMICAL
at a Vpip=-4OmV
current
increases
when the
AND BIOPHYSICAL
PO changes
from
RESEARCH COMMUNICATIONS
0.85
to
0.3
and
the
unitary
of 80%.
QISCUSSION The
aim of
channel
experiments
activity.
amount Ca2+
our
Two facts
of extracellular Kt
The
variation
physiological of Ca ”
zation
from
[Ca*+ Ii
the
um channels of
is
in
experimental
the
rise,
cells
rapidly
of K+- channels allows
and
(see
Fig.
were
obtained
fura-
in
iB1,
depletion
lar
space.
and the
to
as
already
when
using
shows of
A clear
different
that
clamp
time
are
[Ca’+Ii
for
other
ionophore
A23187
evokes
stores was observed levels
instead
(see
of
a marked and to
between Fig. 1433
2B).
not
presence
of
(8.9)
or
influx
the
activity
cells,
of
these
of
Similar
of from of
chan-
the
level
the
may
activity
which
the
changing
the
observed
on the
for
and
a [Ca2+lo
the
(11-131.
transient
voltage cells
excitable
to
types
blocker
were
conductance
of calci-
active”
channels”
cell
of the
following
effect
related
within
through
these
“tonically
The
strictly
in
in
of
elevation
are
However,
has a significant
recordings.
[Ca2+Io
changes
found
of
changes
( an aspecific
of Ca 2+,
as “maxi-K+
shown an
(10)
the
a class
sustained
ICa’+Ii
the
that
of Ca*+ mobili-
channels
verapamil.
K*-
as a consequence
detectable
The entry
example
[Ca’+ Ii
intracellular link
no
channels”
in
patch
open
fact,
and
be classified
the
response
the
our
them
probability
“fast rise
not
of
seems to occur
calcium
is
by KCl.
as for
by
but
entry
channel
by nifedipine
modulated
as a result
a little
these
In
that
by 3pM La3+
Apparently,
inactivating
and not
Only
second,
only
on the
first,
increase
occur
inhibited
depolarized
The
to
space
of
are an
[Ca’+Ii
results:
and,
and
The calcium
of Ca 2+ -channels,
be hypothesized.
nels
(7).
type
blocked
[Ca’+Ii
appears
of
present
following
conditions.
were
was not
some types the
as this
by the
stores.
(7)).
(WCs)
these
[Ca’+Iit
completely
channels
an influence
present
extracellular
observed
operated
when
of
the
as it
calcium
are
intracellular
has been
proved
(O.l-2mM).
from
prove
modifies
channels
limits
entry
are
calcium
activated
ICaZ+lis
was to
open
[Ca’+Ii results
[Ca2+Io.
[Ca2+Ii, the the
The due to
extracelluK+channels
Vol.
182,
All
No.
these in
channels is
are
It
growth
is
the
clearly
present
that
(14).
Although
&Q
membrane
and tissue
not
only
(D.l-2mM),
potential
that
total
these
calcium
as a function these
situation,
cart i lage , may influence cyte
BIOPHYSICAL
RESEARCH
that but
the
also
COMMUNICATIONS
lCa’*li
that
depends
CaZt-activated
on Kt
in chondrocytes.
varies
b
range
to hypothesize known
AND
demonstrate
physiological
plate,
surface to
the
tempting
tion.
BIOCHEMICAL
results
[Ca2+lo
It
3, 1992
the the
(11,
the
on cell
in
from
can only
existing
conductances
with
in calcifica-
different the
in part
gradient,
differentiation,
a role the
distance
studies
calcium membrane
may play
concentration, of
in vitro
changes
zones
mineralization be extrapolated
Jo w an
matrix
of
effect vesicle
in on
growth chondro-
formation
calcification.
ACKNOWLEDGMENTS This work Miss M.T. Fondo per ter, and scapulas.
was supported by research grants from CNR and MURST, Italy. We thank Nicodemo for her valid technical assistance. We also acknowledge the lo Studio delle Malattie de1 Fegato for use of the spectrofluoromethe Uanetto Delicatessen Factory for the generous supply of pip
REFERENCES 1.
2. 3. 4. 5. 6. 7. a. 9. ::: 12. 13. 14.
Edelman. A., Thil, C.L., Garabedian, M., Plachot, J.J., Guillozo, H., Fritsch, J., Thomas, S.R., Balsan, S. (1985) Min. Electr. Metab. 11,97-105. Grinstein, S. and Dixon, S.J. (1989) Physiol. Rev. 69.417-481. Crandolfo, M.. Martina, M., Ruzzier, F., Vittur, F. (1990). Calcif. Tissue Tnt. 47, 302-307. Vittur, F., Pugliarello, M.C., de Bernard, B. (1971) Experientia 27,126-127. D’Andrea, P., Grandolfo, M.. de Bernard, 6. Vittur, F. (1990) Exp. Cell Res. 191, 22-26. Meldolesi I J., Huttner, W.B., Tsien, R.Y., Pozzan, T. (1984) Proc . Nat. Acad. Sci. USA 81,620-624. Nemeth, E.F. (1990) Cell Calcium 11.323-327. Benham, C.D. and Tsien, R.W. (1987) in Cell calcium and the control of membrane transport (L. J. Mandel, D.C. Eaton, Eds), pp 45-64. The Rockefeller University Press, New York. Rosenberg, R.L., Hess, P., Tsien. R.W. (1988) J. Gen. Physiol. 92.27-54. Meldolesi, J. and Pozzan, T. (1987) Exp. Cell Res. 171, 271-283. Latorre, R.. Vergara M.C., Hidalso, C. (1982) Proc. Natl. Acad.Sci. USA 79.805-809. Schwarz, W.and Passow, H. (1983) Ann. Rev. Physiol. 45.359-374. Latorre. R., Oberhauser, A.. Labarca, P.. Alvarez, 0. (1989) Ann. Rev. Physiol. 51.385-399. Howell, D.S., Delchamps, E., Riemer. W., Kiem, I. (1960) J. Clin. Invest. 39.919-929. 1434