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The Journal of Neuroscience, November 1, 1998, 18(21):8605-8613
Low-Voltage-Activated Ca2+ Currents Are Generated by
Members of the CavT Subunit Family ( 1G/H) in Rat Primary
Sensory Neurons
Régis C.
Lambert1,
Frank
McKenna1,
Yves
Maulet1,
Edmund M.
Talley2,
Douglas A.
Bayliss2,
Leanne L.
Cribbs3,
Jung-Ha
Lee3,
Edward
Perez-Reyes3, and
Anne
Feltz1
1 Laboratoire de Neurobiologie Cellulaire, UPR
9009-Centre National de la Recherche Scientifique, F-67084, Strasbourg,
France, 2 Department of Pharmacology, University of
Virginia, Charlottesville, Virginia 22908, and 3 Loyola
University Medical Center, Maywood, Illinois 60153
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ABSTRACT |
Recently, two members of a new family of Ca2+
channel  1 subunits, 1G (or CavT.1) and 1H (or
CavT.2), have been cloned and expressed. These 1
subunits generate Ba2+ currents similar to the
T-type Ca2+ currents present in sensory neurons.
Here, we use three methods to investigate whether the T currents of
nodosus ganglion neurons are encoded by members of the CavT
family. PCR detected the presence of mRNA encoding both 1G
and 1H, as well as a third highly related sequence, 1I. In
situ hybridizations performed on nodosus ganglia demonstrate a
high expression of 1H subunit RNAs. Transfection of nodosus ganglion
neurons with a generic antisense oligonucleotide against this new 1
subunit family selectively suppresses the low-voltage-activated
Ca2+ current. The antisense oligonucleotide effect
increased with time after transfection and reached a maximum 3 d
after treatment, indicating a 2-3 d turnover for the 1 proteins.
Taken together, these results suggest that the T-type current present
in the sensory neurons is mainly attributable to 1H channels. In
addition, taking advantage of the high specificity of the antisense ON
to the cloned channels, we showed that T-type currents greatly slowed
the repolarization occurring during an action potential and were
responsible for up to 51% of the Ca2+ entry during
spikes. Therefore, the antisense strategy clearly demonstrates the role
of low-voltage-activated Ca2+ current in affecting
the afterpotential properties and influencing the cell excitability.
Such tools should be beneficial to further studies investigating
physiological roles of T-type Ca2+ currents.
Key words:
low-threshold/T-type calcium channels; antisense
oligonucleotides; PCR; in situ hybridization; action
potentials; sensory neurons; nodosus ganglion
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INTRODUCTION |
The existence of a neuronal
Ca2+ current elicited just above the resting
potential was first established in primary sensory neurons (Carbone and
Lux, 1984a ; Bossu et al., 1985; Fedulova et al., 1985; Nowycky et al.,
1985). Consequently, many properties of the low-voltage-activated (LVA)
or T-type Ca2+ currents have been described in this
cell type. Briefly, LVA channels have a 8-10 pS conductance in either
20 mM Ca2+ (Carbone and Lux, 1984a) or
100 mM Ba2+ (Fox et al., 1987b).
Resulting whole-cell currents are transient, activating approximately
 60 mV, with complete steady-state inactivation above 50 mV (Nowycky
et al., 1985; Bossu and Feltz, 1986; Carbone and Lux, 1987; Fox et al.,
1987a,b). In contrast to high-voltage-activated (HVA)
Ca2+ currents, T-type currents display slow
deactivation (Carbone and Lux, 1984b; Armstrong and Matteson, 1985;
Matteson and Armstrong, 1986). Despite the fact that detailed studies
are greatly impeded by the lack of a specific pharmacology, the unique
properties of LVA currents implicate these channels in many
physiological functions. More specifically, in neurons they have been
suggested to be responsible for repetitive firing activity, intrinsic
neuronal oscillations, and Ca2+ entry during spikes
(for review, see Huguenard, 1996).
Many efforts have been devoted to the molecular characterization of LVA
channels. Until recently, no cloned Ca2+ channel
1 subunit was shown to generate current with properties similar to
the LVA currents. However, this year two studies have offered a
distinct hypothesis to account for the molecular counterpart of the
T-type current. Meir and Dolphin (1998) have reported in COS7 cells
that expressed 1B, 1C, and 1E subunits (Snutch et al., 1990;
Soong et al., 1993; Schneider et al., 1994), which classically generate
HVA currents, can also form small conductance channels with properties
similar to native T-type channels. On the other hand, the Perez-Reyes
laboratory has reported cloning and characterization of a new 1
subunit family, called CavT (Cribbs et al., 1998;
Perez-Reyes et al., 1998a). The two members of the family expressed so
far, the 1G (or CavT.1) and 1H (or
CavT.2) subunits, encode currents displaying
biophysical properties similar to the LVA Ca2+
current of sensory neurons. In a first attempt to clarify the molecular
counterpart of the LVA Ca2+ channel in
situ, we have shown previously, using an antisense oligonucleotide
(ON) strategy, that depletion of the Ca2+ channel
auxiliary  subunit specifically affects HVA current properties
without modifying LVA current properties in nodosus ganglion neurons
(Lambert et al., 1997). However, this observation does not make it
possible to choose which 1 family encodes T-type channels in sensory
neurons. Indeed, small-conductance HVA channel properties are not
sensitive to coexpression of the subunit (Meir and Dolphin, 1998),
and CavT subunits have low sequence homology (~30%
similarity) with other Ca2+ channel subunits,
lacking the AID sequence (Perez-Reyes et al., 1998a) in the
intracellular loop I-II where subunits bind with high affinity
(Pragnell et al., 1994). Therefore, we have extended our in
situ studies to finally identify the 1 subunit underlying T-type current in sensory neurons. We show here that an antisense ON
designed against the CavT subunit family (Perez-Reyes et
al., 1998b) suppresses the T-type current in nodosus ganglion neurons. In addition, using this highly specific tool to selectively remove the
LVA component of the Ca2+ current, we emphasize the
role of T-type channels in shaping the action potential and determining
the amount of Ca2+ flowing into cranial sensory
neurons during a spike.
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MATERIALS AND METHODS |
Cell culture and transfection. Culture method of rat
nodosus ganglion neurons has been described previously in detail in
Bossu et al. (1985) and briefly reported in Lambert et al. (1997).
Three days after plating, cells were transfected using polyethylenimine (50 kDa; Sigma, St. Louis, MO) as transfecting agent (Lambert et
al., 1996). Cells were exposed for 4 hr to 300 nM
5'-fluorescent antisense ON or 5'-fluorescent scrambled ON (see Table
1 for sequences). Antisense ONs were
designed against the motif NMFVGVVE of DIIISVI, using the nucleotide
sequences of 1G [Perez-Reyes et al. (1998a); GenBank AF027984],
1H [Cribbs et al. (1998); GenBank AF051946], and 1I (GenBank
AL008716). ON had phosphorothioate linkages in all positions.
Reverse transcription-PCR. Fragments of cDNA were amplified
by the PCR after reverse transcription (RT-PCR) [reverse transcriptase from Life Technologies (Gaithersburg, MD)] of
poly(A+) RNA from cultured nodosus ganglion cells
and NIE-115 neuroblastoma cells. First-strand cDNA was synthesized in
the presence of 0.3 µg poly(A+) RNA. The
amplification procedure was as follows: 1 cycle at 94°C for 30 sec;
10 cycles composed of 30 sec at 94°C, 30 sec at 58°C, and 30 sec at
71°C; and 23 cycles composed of 20 sec at 94°C, 30 sec at 58°C,
and 30 sec at 71°C. See Table 1 for primer sequences.
In situ hybridization. Sprague Dawley rats of different
postnatal ages (P0, P7, and adult) were anesthetized either by
hypothermia (P0) or by using a mixture of ketamine and xylazine ( P7).
Nodosus ganglia were removed, and 10 µm sections were thaw-mounted
onto glass slides. Antisense ON 33 bases in length were labeled with [33P] dATP using terminal deoxynucleotidyl
transferase (Life Technologies). Prehybridization, hybridization, and
wash conditions were identical to those described previously (Talley et
al., 1997).
We used multiple ON probes corresponding to the region of the three
genes that encodes the I-II intracellular loop of the channels. The
sequences of the antisense probes are given in Table 1. Each probe was
tested separately on rat brain sections (data not shown); after this
initial characterization the probes for each gene were hybridized to
nodosus ganglia as a mixture, resulting in an enhanced signal.
Specificity of the probes was affirmed by virtue of two separate
findings. First, each probe individually exhibited a restricted CNS
distribution that was identical to that shown by the other probes to
that same gene and, at the same time, distinctly different from the
distributions obtained with probes to the other two genes (our
unpublished observations). Second, concurrent incubation of the
sections with 500- to 1000-fold excess unlabeled oligonucleotide (1 µM) in a competition experiment resulted in complete
elimination of hybridization signal. Five animals were used for each
age group. Hybridized sections were apposed to autoradiographic film
and also dipped in liquid emulsion (NTB2, Kodak).
Antisense experiments in Xenopus oocytes. The rat
brain 1G cDNA (Perez-Reyes et al., 1998a) was subcloned into
pGEM-HEA (a gift from Kenton Swartz, National Institutes of Health),
which contains the 5' and 3' untranslated regions from
Xenopus globin (Liman et al., 1992). Capped cRNA was
synthesized from plasmid linearized with AflII using the T7
mMessage mMachine kit (Ambion, Austin, TX). Cloning and expression of
the human 1E cDNA has been described previously (Schneider et al.,
1995). Oocytes were prepared from Xenopus laevis (NASCO, Ft.
Atkinson, WI) using standard techniques (Bernal et al., 1997). Each
oocyte was injected with 10 ng of cRNA in a volume of 50 nl.
Oligonucleotides were mixed with the cRNA to achieve a final
concentration of 10 µM. Oocytes were incubated at 18°C
for at least 5 d before recording. The ON had no significant
effect on cell viability.
Oocytes were voltage-clamped using a two-microelectrode voltage-clamp
amplifier (OC-725B, Warner Instrument, Hamden, CT). The bath solution
contained the following (in mM): 10 Ba(OH)2, 80 NaOH, 1 KOH, and 5 HEPES, adjusted to pH
7.4 with methanesulfonate. Voltage and current electrodes (1.5-1.8
M tip resistance) were filled with 3 M KCl. Data were
acquired at 4 kHz using the pCLAMP system [Digidata 1200 and pCLAMP
6.0, Axon Instruments (Foster City, CA)] and filtered at 1 kHz.
Electrophysiology of nodosus ganglion neurons. Transfected
cells were identified by their nuclear fluorescence using conventional fluorescence microscopy. Currents/voltages were recorded using an
Axopatch 200A amplifier and pClamp6 software (Axon Instruments) in the
whole-cell configuration of the patch-clamp technique. A minimal 75%
compensation of series resistance (typically 10 M) and capacity
current was achieved. Leak currents were removed by use of a
hyperpolarized P/4 substraction protocol.
Estimation of Ca2+ current density.
Current traces were recorded using a sampling frequency of 10 kHz and
analyzed after filtering at 1 kHz with a digital Gaussian filter.
Ca2+ currents were recorded in isolation by the use
of bath and pipette solutions that maximally reduced the
Na+, K+, and
Cl currents. The bath solution contained (in
mM): 10 CaCl2, 110 trichloroacetate, 10 HEPES, 10 tetraethylammonium chloride, and 10 glucose, adjusted to pH
7.4 with Tris-base. Tetrodotoxin (TTX) was added at a concentration of
1 µM to the extracellular medium to eliminate any
contamination of current flowing through Na+
channels. The pipette solution contained (in mM): 95 HEPES,
3 CaCl2, 30 EGTA, 5 NaCl, 1 MgATP, and 0.2 GTP,
adjusted to pH 7.2 with CsOH. Cell capacitance was estimated from the
time constant of the decay phase of a transient (sampled at 100 kHz,
low-pass-filtered at 10 kHz) elicited by a 5 mV hyperpolarizing step
from a holding potential of 80 mV. In each cell, current density was
measured by constructing several I-V curves with
successive 200 msec depolarizing steps ranging from 60 to 50 mV (5 mV
increments) from a holding potential of 80 mV.
Generation of spikes. Spikes were recorded at a sampling
frequency of 100 kHz (low-pass filter: 10 kHz) and generated by a 1 msec current injection. In this condition, action potential developed a
few milliseconds after the end of the initial depolarization induced by
the current injection, therefore with minimal alteration of the spike
waveform induced by the current injection. The extracellular solution
contained (in mM): 137 NaCl, 2.7 KCl, 2 MgCl2, 2.8 CaCl2, 10 HEPES, and
5.6 glucose; pH was adjusted to 7.4 with TrisOH. The pipette solution
contained in (mM): 125 potassium methylsulfate, 10 sodium
methanesulfonate, 4 KCl, 1 MgCl2, 1 EGTA/KOH, 10 HEPES, 1 MgATP, and 0.5 GTP; pH was adjusted to 7.2 with TrisOH.
Ca2+ entry during action potential. To
estimate Ca2+ entry during the spike, stereotypical
template action-potential waveforms were generated by averaging
recorded spikes synchronized at time of peak amplitude. These templates
were used to evoke Ca2+ currents recorded at 100 kHz
(low-pass filter: 10 kHz). The intracellular medium was identical to
the one used to estimate Ca2+ current density, but
the extracellular medium was modified to impose a more physiological
Ca2+ concentration. The bath solution contained (in
mM): 2.8 CaCl2, 120 trichloroacetate, 10 HEPES, 10 tetraethylammonium chloride, 10 glucose; adjusted to pH 7.4 with Tris-base. TTX was added at a concentration of 1 µM.
Data reported are mean ± SEM.
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RESULTS |
CavT subunits are expressed in nodosus
ganglion neurons
The RT-PCR technique was used to confirm the presence of
CavT subunit RNAs in nodosus ganglion neurons. RNA
fragments ~490 bp long were amplified (Fig.
1), which correspond to 1G (492 bp
long), 1H (489 bp long), and 1I (474 bp long) subunit RNAs. Individual clones from RT-PCR products were sequenced and at least one
clone from each gene was found.
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Figure 1.
CavT RNAs are transcribed in nodosus
sensory neurons. Fragments ~490 bp long can be amplified from nodosus
ganglion cells neurons (lane III;
poly(A+) RNA 0.3 µg) using PCR primers specific
for the newly cloned family of Ca2+ channel
1 subunits (see Table 1). The same size of PCR products
could be amplified approximately to the same extent from
undifferentiated NIE-115 neuroblastoma cells (lane IV;
poly(A+) RNA 0.3 µg), which display prominent
T-type currents (Perez-Reyes et al., 1998a). Lane I is
the 100 bp size marker. Lane II is a negative control
obtained when omitting the reverse transcriptase.
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Antisense ON knock-out of T-type channels in nodosus
ganglion neurons
To investigate further the possible involvement of this family of
1 subunits in generating LVA currents in sensory neurons, an
antisense ON strategy was performed using a generic antisense ON
sequence directed against the DIIISVI domain of the
CavT channels. The ability of the antisense ON to
block channel protein expression was first tested using the
Xenopus laevis system. As reported previously (Perez-Reyes
et al., 1998a), T-type currents can be readily measured from oocytes
injected with 1G cRNA. Channel expression was almost completely
blocked by coinjection of 1G cRNA with the antisense ON (Fig.
2). Small T-type currents (13 nA) were
detected in 2 of 28 oocytes. In contrast, the scrambled ON did not
block expression of T-type currents. The specificity of the antisense
ON was tested by coinjecting it with 1E cRNA into oocytes. Typical
high-voltage-activated currents were measured from both oocytes
injected with either 1E or 1E plus antisense ON (data not shown;
n = 6).
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Figure 2.
Antisense, but not scrambled ON block expression
of 1G in Xenopus oocytes. Oocytes were injected with
either 1G (n = 14), 1G plus antisense ON
(n = 28), or 1G plus scrambled ON
(n = 20). The results were obtained from oocytes
from three frogs. Currents were recorded during test pulses to 20 mV
from a holding potential of 90 mV.
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The same antisense and scrambled ON were further used in nodosus
ganglion neuron cultures. In antisense and scrambled ON-transfected neurons, Ca2+ currents were recorded using 10 mM Ca2+ as the ion charge carrier to
maximally separate low- and high-voltage-activated currents.
Transfected cells were distinguished by the use of
fluorescein-conjugated ON, whose intracellular presence induced a
strong staining of the cell nucleus [for details, see Lambert et al.
(1996)]. To avoid culture-to-culture and transfection-to-transfection
variability, and to assess any nonspecific effect of ON transfection on
the membrane properties of the cells, scrambled ON-transfected neurons were recorded in each experiment as controls. Using this methodology, we observed that depletion of the CavT subunits induced a
dramatic decrease in LVA current amplitude (Fig.
3A). Comparison of mean current densities measured 3 d after treatment in both groups of
neurons indicated that almost no LVA Ca2+ current
could be evoked in antisense ON-transfected cells. By contrast, no
effect on the HVA current density was observed (Fig. 3B). To
confirm the absence of antisense ON effect on HVA currents, Boltzmann
functions (I = G (V Erev)/(1 + exp[(V V0.5)/k])) were fitted to
I-V curves constructed from the amplitude of the Ca2+ currents measured at the end of 200 msec
depolarizing steps (data not shown). The fast inactivation properties
of T-type channels ensure that such Ca2+ currents
are attributable solely to the activation of HVA channels. This
procedure was used to describe the characteristics of the mixed
population of HVA channels, with no difference being observed in mean
parameter values of the Boltzmann fits: G = 0.54 ± 0.07 and 0.49 ± 0.05 pS/pF; V0.5 = 17.4 ± 0.7 and 16.0 ± 0.6 mV; k = 5.7 ± 0.2 and 5.4 ± 0.3; Erev = 77.0 ± 1.5 and 73.3 ± 1.4 mV in antisense (n = 11) and
scrambled (n = 14) ON-transfected cells, respectively.
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Figure 3.
Antisense ON reduces the LVA
Ca2+ current with no effect on HVA currents.
A and B show typical currents recorded in
antisense (A) and in scrambled
(B) ON-treated cells depolarized with 200 msec
steps either to 20 mV (top trace) or +30 mV
(bottom trace) from 80 mV holding potential. Note that
the antisense ON-treated cell displayed almost no LVA current. Cells
were from the same culture and recorded 3 d after transfection. In
C, current density-voltage relationships of peak
current show a dramatic reduction of LVA current 3 d after
transfection in antisense ON-treated cells when compared with scrambled
ON-transfected cells.
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To characterize the progression of the antisense ON effect, a
systematic study of Ca2+ current densities was
performed every day after transfection. Maximal T-type current
densities were measured at 20 mV, thus allowing LVA currents to be
recorded in isolation. Maximal HVA current densities were estimated
from current amplitude obtained at the end of 200 msec depolarizing
steps. The antisense ON effect was detectable the first day after
treatment and increased thereafter (Fig.
4A). A maximum decrease
of 78.7 ± 2.2% (n = 11) in LVA current density
was achieved 3 d after transfection, suggesting a turnover time of
2-3 d for these 1 subunits (Fig. 4B).
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Figure 4.
T-type and HVA current densities as a function of
time after transfection. In A, right and
left histograms refer to HVA and LVA mean current
densities, respectively. HVA current densities were estimated from
maximal current obtained after 200-msec-long depolarizations. Peak
current amplitudes observed at 20 mV were used to calculate T-type
current densities. Averaged data from antisense ON-transfected neurons
are shown in black bars. Averaged data obtained from
scrambled ON-transfected neurons are shown in white
bars. Numbers of cells are indicated inside each bar in the HVA
mean current density histogram (left histogram). Note
that the current densities of the HVA channels are similar in both
groups and that the T-type current is reduced in cells treated with
antisense ON as compared with cells treated with scrambled ON. In
B, current densities observed in antisense
ON-transfected cells were expressed as percentage of the mean current
densities calculated for scrambled ON-treated neurons. Antisense ON
effects on HVA ( ) and LVA ( ) current densities were reported as a
function of the time after transfection. Numbers of cells are indicated
in brackets.
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In conclusion, this study clearly demonstrates that the newly cloned
family of 1 subunits is responsible for the T-type currents in
nodosus ganglion sensory neurons.
Expression of genes encoding T-type calcium channels in nodosus
ganglion neurons
To determine which member of the CavT subunit family
is responsible for the LVA Ca2+ current, in
situ hybridization was used to identify the 1 subunit RNAs
present in nodosus ganglion neurons. We hybridized a mixture of
[33P]-labeled ON corresponding to each of the
three known members of the CavT family of genes. At each of
the different ages tested (P0, P7, and adult), an intense signal was
generated by probes specific to the 1H gene, whereas probes specific
to the 1G and 1I genes generated signals that were much weaker
(Fig. 5). Visualization of silver grains
from emulsion-dipped slides revealed that mRNA for 1G was present at
low levels in many neurons, with scattered neurons exhibiting a
moderate signal. On the other hand, labeling for 1I was detectable
above background [as assessed in competition experiments using excess
amounts of unlabeled ON (data not shown)] in only a few neurons.
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Figure 5.
In situ hybridization reveals
expression of 1G, 1H, and 1I Ca2+ channel
subunits in nodosus ganglion neurons. Ganglia were dissected from
7-d-old rats, hybridized with 33P-labeled oligonucleotides,
and exposed to autoradiographic emulsion. Low-power dark-field images
are shown on the left (A, C, and
E); high-power bright-field images are shown on the
right (B, D, and
F). In each pair of micrographs, the same labeled
neuron is indicated by arrows. Uniformly high expression
was seen for the 1H subunit (C, D). 1G expression
also was uniform, but the intensity of the labeling was much lower
(A, B), with the exception of scattered neurons that
were moderately labeled (arrows). Labeling for the 1I
subunit was detectable only in a few neurons (E, F,
arrows). Scale bar (shown in F):
A, C, E, 40 µm; B, D, F, 10 µm.
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Effect of T-type channel depletion on
action-potential waveform
Given that a very specific suppression of LVA current could be
obtained by antisense ON treatment, we applied this technique to study
the role(s) of LVA Ca2+ currents in sensory neurons.
Because the conductance and activation-deactivation properties of
T-type currents suggest that they may contribute to
Ca2+ entry during the action potential, we first
compared spikes generated in either antisense or scrambled ON-treated
neurons using extra and intracellular solutions close to physiological
conditions [mainly 137 mM NaCl and 2.8 mM
Ca2+ in the extracellular medium (see Materials and
Methods)]. Averaged action-potential waveforms obtained 3 d after
transfection show a slower repolarization when T-type channels are
expressed [scrambled ON-treated neurons (Fig.
6)] compared with cells devoid of LVA channels (antisense ON-transfected neurons). Because LVA currents can
be fully activated from hyperpolarized potentials, the slowing of the
repolarization phase was observed only in spikes generated from 80 mV
holding potential (compared with 60 mV holding potential), which
confirms the role of T-type current in this phenomenon. Under these
conditions, T-type currents induced a final long-lasting depolarizing
component (Fig. 6, star in bottom traces) in
addition to a broadening of the waveform.
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Figure 6.
Role of the T-type current in shaping the
action-potential waveform. Spikes were generated in antisense
(bold traces) and scrambled (faint
traces) ON-treated neurons. Traces show averaged waveforms
obtained at two potentials: 60 mV (top traces) and
80 mV (bottom traces). The 60 mV potential is close
to resting potential and results in partial steady-state inactivation
of the T-type current. Note that in this case antisense and scrambled
ON-treated cells generate almost identical waveforms. At 80 mV, full
activation of T-type current is made possible. In this latter
condition, spikes recorded in scrambled ON-treated cells were slower
and further prolonged by a depolarizing tail potential absent in
antisense ON-treated cells. Student's t test was
performed on values obtained at time indicated by the
star. Difference is significant with
p < 0.008.
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Role of T-type currents in Ca2+ entry
during spikes
The average action-potential waveform obtained in scrambled
ON-transfected neurons was used as a template to depolarize the cells
and evoke Ca2+ current in voltage-clamp protocols.
In these experiments, Ca2+ currents were recorded
with a more physiological extracellular Ca2+
concentration of 2.8 mM, equal to the one used when
recording spikes. The reduced divalent ion concentration, as compared
with the 10 mM concentration used previously during
description of the antisense ON effect, decreased the T-type current
amplitude. Three days after transfection, mean current density
evaluated at 20 mV in scrambled ON-treated cells was 4.8 ± 1.7 pA/pF (n = 6) in 2.8 mM
Ca2+ and 10.2 ± 1.1 pA/pF (n = 19) in 10 mM Ca2+. The decrease in
extracellular Ca2+ induced a 13 mV hyperpolarizing
shift in the activation potential of the HVA currents (in 2.8 mM Ca2+, Boltzmann fit parameters were
G = 0.39 ± 0.22 pS/pF;
V0.5 = 4.4 ± 2.5 mV; k = 5.7 ± 1.4; and Erev = 59.1 ± 5.1 mV;
n = 9). In these conditions, Ca2+
entry during spikes could be compared between neurons transfected with
antisense ON (consequently displaying no T-type current) and neurons
treated with scrambled ON. As illustrated in Figure 7, the presence of LVA channels
dramatically modifies Ca2+ currents recorded during
the template action potentials. T-type channel activation induces a
late Ca2+ current clearly distinguishable from the
HVA currents and is responsible for half of the Ca2+
entry during spikes. Indeed, by subtracting and integrating averaged traces obtained 3 d after transfection in neurons treated with antisense or scrambled ON (Fig.
8A), it was calculated
that ~50.8% of the Ca2+ entry was attributable to
LVA current in scrambled ON-transfected cells. Finally,
Ca2+ tail currents were generated at different times
during the spike to measure the level of Ca2+
channel activation, which otherwise cannot be directly estimated from
the Ca2+ current traces because of continuous
variation of the driving force. A series of templates designed to
depolarize neurons for different time intervals of the action-potential
waveform were applied to scrambled and antisense ON-transfected cells
(Fig. 8B). The tail current amplitudes observed at
different times during spikes indicate that T-type channel activation
is not evident early in the action potential. On the other hand, slower
kinetics of tail currents recorded in scrambled ON-treated cells
clearly reflect the presence of LVA channels. Surprisingly, in both
groups of neurons, the activation of the Ca2+
channels is maximal around the peak of the spike. This suggests that
although significant Ca2+ entry occurs during spike
repolarization, the Ca2+ channels may participate in
spike depolarization by increasing the membrane conductance.
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Figure 7.
Ca2+ entries during spikes.
Waveforms obtained by averaging spikes generated in scrambled
ON-treated cells were used to depolarize scrambled
(A) and antisense (B)
ON-treated neurons. Top traces show the voltage template
and bottom traces show the Ca2+
current at 60 and 80 mV resting potentials, respectively.
Insets illustrate the presence of T-type currents in the
scrambled ON-transfected neuron and its absence in the antisense
ON-treated neuron. Note in this latter case the absence of late
Ca2+ current during spike. In contrast, a late
Ca2+ component is observed in
A.
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Figure 8.
Mean Ca2+ current and tail
currents during an action potential. In A, averaged
Ca2+ currents were recorded by depolarizing
scrambled (thin trace, n = 6) and
antisense (thick trace, n = 7)
ON-transfected neurons from 80 mV holding potential using a spike
template (top trace). Note the late
Ca2+ entry present in scrambled ON-treated neurons.
Student's t test was performed on values obtained at
time indicated by the star. The difference is
significant with p < 0.005. B
illustrates traces obtained when depolarizing either an antisense ON
(bottom traces) or scrambled ON (middle
traces)-transfected neurons with successive spike templates
repolarized to 80 mV at an increasing time interval (top
traces). Note in both cells the similar pattern of tail current
amplitudes at the beginning of the spike, with clear differences only
in the late component of the action potential. However, a slow
component in the tail kinetics, attributable to the slow deactivation
of T-type channels, can be seen in scrambled ON-treated cells. Note
also that Ca2+ channels are opened very early during
the spike (depolarizing phase), although a Ca2+
entry occurred mainly during the repolarizing phase.
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In conclusion, specific knock-out of T-type channels with antisense ON
emphasizes the major role of this LVA current in both shaping the
action-potential waveform and determining the amount of
Ca2+ flowing into sensory neurons during a
spike.
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DISCUSSION |
Properties of the recently cloned pore forming 1G [or
CavT.1 (Perez-Reyes et al., 1998a)] and 1H [or
CavT.2 (Cribbs et al., 1998)] subunits make these proteins
good candidates for the T-type channels in primary sensory neurons. We
presently show that a generic antisense ON sequence designed against a
motif of the DIIISVI segment common to all the CavT
channels family actually abolishes T-type current in this cell type. A
more precise identification of the 1 subunit responsible for the LVA
Ca2+ current in sensory neurons will be possible
when specific antibodies become available. However, a partial answer to
this question was obtained by carrying out in situ
hybridization.
The fact that the hybridization signal corresponding to 1H was seen
at a much higher intensity relative to that of 1G and 1I prompts
the interpretation that this transcript may be present in greater
abundance than the other two species of mRNA. It is important to point
out, however, that in situ hybridization is only
semi-quantitative, and factors other than expression levels (such as
hybridization efficiency of the individual probes) can influence signal
intensity. Nevertheless, for each transcript, multiple probes (of
identical length and similar GC content) individually generated
signal intensities that were consistent across all of the brain regions
examined (our unpublished observations). This consistency
between probes recognizing the same transcript suggests that the
influence of factors such as differences in hybridization efficiency
are minor and that variations in signal intensity primarily reflect
mRNA accumulation. Therefore, given that the hybridization signal for
1H is far more intense than the signal for 1G or for 1I, it is
likely that 1H indeed represents the most prevalent transcript in
nodosus neurons.
Reciprocally, when considering data obtained by functional expression
of 1G and 1H subunits in Xenopus oocytes (Perez-Reyes et al., 1998a) and HEK293 cells (Cribbs et al., 1998), respectively, it
is clear that the biophysical properties of the resulting currents are
close to that of the T-type current in sensory neurons (voltage dependence, current kinetics, conductance). In addition, both 1G and
1H subunits have no AID motif for subunit binding (Pragnell et
al., 1994; Perez-Reyes et al., 1998a), and in contrast to other Ca2+ channel 1 subunits (HVA subunits), a high
expression of 1 subunit proteins is obtained in absence of any
auxiliary subunit. This is in agreement with our previous observation
that T-type channels in nodosus ganglion neurons are not affected by
subunit depletion [Lambert et al. (1997), but see Lacerda et al.
(1994)]. However, to complete the full comparison between 1G/H
subunits and LVA Ca2+ channels in sensory neurons,
other criteria such as the blocking effect of divalent ions (Carbone
and Lux, 1987; Fox et al., 1987a) and the sensitivity to amiloride
(Tang et al., 1988) have to be examined.
In the final part of our work we have exploited the selective knock-out
of T-currents to examine their contribution to the shaping of the spike
waveform and the control of Ca2+ entry during action
potentials. Previously, taking advantage of the relatively specific
effect of amiloride on T-type currents in dorsal root ganglion neurons,
McCobb and Beam (1991) and Scroggs and Fox (1992) examined the
contribution of LVA and HVA channels to Ca2+ influx
during a spike. Indeed, the direct knock-out of T-type channels in the
cells used in the present study yields similar estimates. In the
presence of 2 mM extracellular Ca2+ and
when the holding potential is fixed to 80 mV to maximally recruit
T-type channels, LVA current accounts for half of the Ca2+ entry during the time of a spike, with HVA
currents accounting for the other half. In addition, we also examined
the timing of the openings of the various Ca2+
channels and the influence of the T-type current on the shaping of the
action-potential waveform. The amplitude of the tail currents obtained
after stepping back to 80 mV at various times along the spike
waveform yields an estimate of the number of channels that are opened.
Interestingly, in all cases (antisense and scrambled ON-treated cells),
the largest conductance changes occur during the peak of the spike,
which suggests that not only Na+ but also
Ca2+ channels contribute to the peak depolarization.
However, in terms of Ca2+ influx, the maximal
contribution of Ca2+ channels occurs during the
repolarizing phase of the action potential as a consequence of the
increased driving force. During repolarization, the shoulder in the
action-potential waveform is directly related to
Ca2+ inward currents. Because half of the current
can be of T-type origin in the present conditions (close to the
physiological conditions for Ca2+ currents), it is
clear that T-type channels contribute to spike prolongation when they
are activatable. In addition, in cells expressing LVA channels, a pure
T-type current component prolongs the spike after membrane has
repolarized below 60 mV and further contributes to the
Ca2+ entry over the following 10 msec. The
Ca2+-induced permeabilities specific to this cell
type therefore will affect the afterpotential properties and influence
the cell excitability.
In a previous work (Lambert et al., 1997), we have shown that in
nodosus ganglion cells, large T-type current densities are confined to
a subset of large-diameter neurons. This suggests that LVA channels are
likely to have an important role in carrying signals through the
ganglion cells that give rise to the A /A fibers. Our
understanding of temperature or arterial pressure perception and of the
origin of pain (for review, see Scott, 1992) will rely partly on the
identification of the parameters that modulate the contribution of
T-type channels in spike generation.
| |
FOOTNOTES |
Received June 15, 1998; revised Aug. 6, 1998; accepted Aug. 12, 1998.
This work was supported by grants from the National Institute of Heart,
Lung and Blood, HL 57828 (E.P.-R.), National Institutes of Health, NS
33583 (D.A.B.), and the American Heart Association, 96010950 (D.A.B.).
F.M. has an Eli Lilly postdoctoral fellowship.
Correspondence should be addressed to Dr. Régis C. Lambert,
Laboratoire de Neurobiologie Cellulaire, UPR 9009-Centre
National de la Recherche Scientifique, 5 rue B. Pascal, F-67084,
Strasbourg, France.
| |
REFERENCES |
-
Armstrong CM,
Matteson DR
(1985)
Two distinct populations of calcium channels in a clonal line of pituitary cells.
Science
227:65-67[Abstract/Free Full Text].
-
Bernal J,
Lee JH,
Cribbs LL,
Perez-Reyes E
(1997)
Full reversal of Pb2+ block of L-type Ca2+ channels requires treatment with heavy metal antidotes.
J Pharmacol Exp Ther
282:172-180[Abstract/Free Full Text].
-
Bossu JL,
Feltz A
(1986)
Inactivation of the low-threshold transient calcium current in rat sensory neurons, evidence for a dual process.
J Physiol (Lond)
376:341-357[Abstract/Free Full Text].
-
Bossu JL,
Feltz A,
Thomann JM
(1985)
Depolarization elicits two distinct calcium currents in vertebrate sensory neurones.
Pflügers Arch
403:360-368[Web of Science][Medline].
-
Carbone E,
Lux HD
(1984a)
A low voltage-activated, fully inactivating Ca channel in vertebrate sensory neurones.
Nature
310:501-502[Medline].
-
Carbone E,
Lux HD
(1984b)
Low voltage-activated calcium conductance in embryonic chick sensory neurons.
Biophys J
46:413-418[Web of Science][Medline].
-
Carbone E,
Lux HD
(1987)
Kinetics and selectivity of a low-voltage-activated calcium current in chick and rat sensory neurones.
J Physiol (Lond)
386:547-570[Abstract/Free Full Text].
-
Cribbs LL, Lee JH, Yang J, Satin J, Zhang Y, Daud A, Barclay J,
Williamson MP, Fox M, Rees M, Perez-Reyes E 1998 Cloning and
characterization of 1H from human heart, a member of the
T-type calcium channel gene family. Circ Res, in press.
-
Fedulova SA,
Kostyuk PG,
Veselovsky NS
(1985)
Two types of calcium channels in the somatic membrane of new-born rat dorsal root ganglion neurones.
J Physiol (Lond)
359:431-446[Abstract/Free Full Text].
-
Fox AP,
Nowycky MC,
Tsien RW
(1987a)
Kinetic and pharmacological properties distinguishing three types of calcium currents in chick sensory neurones.
J Physiol (Lond)
394:149-172[Abstract/Free Full Text].
-
Fox AP,
Nowycky MC,
Tsien RW
(1987b)
Single channel recordings of three types of calcium channels in chick sensory neurones.
J Physiol (Lond)
394:173-200[Abstract/Free Full Text].
-
Huguenard JR
(1996)
Low-threshold calcium currents in central nervous system neurons.
Annu Rev Physiol
58:329-348[Web of Science][Medline].
-
Lacerda AE,
Perez-Reyes E,
Wei X,
Castellano A,
Brown AM
(1994)
T-type and N-type calcium channels of Xenopus oocytes: evidence for specific interactions with subunits.
Biophys J
66:1833-1843[Web of Science][Medline].
-
Lambert RC,
Maulet Y,
Dupont JL,
Mykita S,
Craig P,
Volsen S,
Feltz A
(1996)
Polyethylenimine-mediated DNA transfection of peripheral and central neurons in primary culture: probing Ca2+ channel structure and function with antisense oligonucleotides.
Mol Cell Neurosci
7:239-246[Web of Science][Medline].
-
Lambert RC,
Maulet Y,
Mouton J,
Beattie R,
Volsen S,
De Waard M,
Feltz A
(1997)
T-type Ca2+ current properties are not modified by Ca2+ channel subunit depletion in nodosus ganglion neurons.
J Neurosci
17:6621-6628[Abstract/Free Full Text].
-
Liman ER,
Tytgat J,
Hess P
(1992)
Subunit stoichiometry of a mammalian K+ channel determined by construction of multimeric cDNAs.
Neuron
9:861-871[Web of Science][Medline].
-
Matteson DR,
Armstrong CM
(1986)
Properties of two types of calcium channels in clonal pituitary cells.
J Gen Physiol
87:161-182[Abstract/Free Full Text].
-
McCobb DP,
Beam KG
(1991)
Action potential waveform voltage-clamp commands reveal striking differences in calcium entry via low and high voltage-activated calcium channels.
Neuron
7:119-127[Web of Science][Medline].
-
Meir A,
Dolphin AC
(1998)
Known calcium channel 1 subunits can form low-threshold small conductance channels with similarities to native T-type channels.
Neuron
20:341-351[Web of Science][Medline].
-
Nowycky MB,
Fox AP,
Tsien RW
(1985)
Three types of neuronal calcium channel with different calcium agonist sensitivity.
Nature
316:440-446[Medline].
-
Perez-Reyes E,
Cribbs LL,
Daud A,
Lacerda AE,
Barclay J,
Williamson MP,
Fox M,
Rees M,
Lee JH
(1998a)
Molecular characterization of a neuronal low-voltage-activated T-type calcium channel.
Nature
391:896-900[Medline].
-
Perez-Reyes E,
Cribbs LL,
Daud A,
Yang J,
Lacerda AE,
Barclay J,
Williamson MP,
Fox M,
Rees M,
Lee JH
(1998b)
Molecular characterization of T-type calcium channels.
In: T-type calcium channels (Nargeot J,
Clozel J-P,
Tsien RW,
eds), pp 290-305. Chester, UK: Adis Press.
-
Pragnell M,
De Waard M,
Mori Y,
Tanabe T,
Snutch TP,
Campbell KP
(1994)
Calcium channel -subunit binds to a conserved motif in the I-II cytoplasmic linker of the 1-subunit.
Nature
368:67-70[Medline].
-
Schneider T,
Wei X,
Olcese R,
Costantin JL,
Neely A,
Palade P,
Perez-Reyes E,
Qin N,
Zhou J,
Crawford GD,
Smith RG,
Appel SH,
Stefani E,
Birnbaumer L
(1994)
Molecular analysis and functional expression of the human type E neuronal Ca2+ channel 1 subunit.
Receptors Channels
2:255-270[Web of Science][Medline].
-
Schneider T,
Perez-Reyes E,
Nyormoi O,
Wei X,
Crawford GD,
Smith RG,
Appel SH,
Birnbaumer L
(1995)
Alpha-1 subunits of voltage gated Ca2+ channels in the mesencephalon x neuroblastoma hybrid cell line MES23.5.
Neuroscience
68:479-485[Web of Science][Medline].
-
Scott SA
(1992)
In: Sensory neurons: diversity, development, and plasticity. New York: Oxford UP.
-
Scroggs RS,
Fox AP
(1992)
Multiple Ca2+ currents elicited by action potential waveforms in acutely isolated adult rat dorsal root ganglion neurons.
J Neurosci
12:1789-1801[Abstract].
-
Snutch TP,
Leonard JP,
Gilbert MM,
Lester HA,
Davidson N
(1990)
Rat brain expresses a heterogenous family of calcium channels.
Proc Natl Acad Sci USA
87:3391-3395[Abstract/Free Full Text].
-
Soong TW,
Stea A,
Hodson CD,
Dubel SJ,
Vincent SR,
Snutch TP
(1993)
Structure and functional expression of a member of the low voltage-activated calcium channel family.
Science
260:1133-1135[Abstract/Free Full Text].
-
Talley EM,
Sadr NN,
Bayliss DA
(1997)
Postnatal development of serotonergic innervation, 5-HT1A receptor expression, and 5-HT responses in rat motoneurons.
J Neurosci
17:4473-4485[Abstract/Free Full Text].
-
Tang C-M,
Presser F,
Morad M
(1988)
Amiloride selectively blocks the low threshold (T) calcium channel.
Science
240:213-215[Abstract/Free Full Text].
Copyright © 1998 Society for Neuroscience 0270-6474/98/18218605-09$05.00/0
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Top
Abstract
Introduction
