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Vol. 59, Issue 5, 1243-1248, May 2001
2
Subunits
Structure and
Gabapentin Binding
Institut für Pharmakologie und Toxikologie der Technischen Universität München, München, Germany
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Abstract |
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 Top
 Abstract
 Introduction
Materials and Methods
Results
Discussion
References
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High-voltage activated calcium channels are modulated by a series of
auxiliary proteins, including those of the 
2
family. Until recently, only a single 2 subunit was known,
but two further members, 2-2 and -3, have since been
identified. In this study, the structure of these two novel subunits
has been characterized and binding of the antiepileptic drug gabapentin
investigated. Using antibodies directed against the amino terminal
portion of the proteins, the gross structure of the subunits could be
analyzed by Western blotting. Similar to 2-1, both
2-2 and -3 subunits consist of two proteins
a larger
2 and a smaller that can be separated by reduction.
The subunits are also highly N-glycosylated with
approximately 30 kDa of their mass consisting of oligosaccharides. 2-1 was detected in all mouse tissues studied,
whereas 2-2 was found at high levels in brain and
heart. The 2-3 subunit was observed only in brain.
2-1 and 2-2, but not
2-3, were found to bind gabapentin. The
Kd value of gabapentin binding to 2-2 was 153 nM compared with the higher affinity
binding to 2-1 (Kd = 59 nM).
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Introduction |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Voltage
gated calcium channels are multisubunit complexes that permit the
influx of calcium ions into cells after changes in the plasma membrane
potential. A number of voltage gated calcium channels exist, which can
be broadly grouped into high-voltage (HVA) and low-voltage activated
(LVA) channels. The HVA channels can be further subgrouped as L-, R-,
P/Q-, and N-type, depending on their biophysical characteristics. The
channels consist minimally of an 1 pore
protein that conducts current, contains the voltage sensor, and is the
target of several drugs. Seven genes have been identified for the
1 subunits of HVA channels and three for LVA channels (for reviews, see Hofmann et al., 1999
; Lacinová et al.,
2000). Although it is known that HVA channels are modulated by
accessory subunits, it remains to be unequivocally established whether
the LVA channels are associated with other proteins. The HVA auxiliary
subunits are 
(four genes), 2 (three),
and 
(six). Most of these subunits have splice variants, giving rise to an even larger number of possible channel combinations and behaviors. Mutations of several channel proteins have been shown to be
a causative factor in neurological disorders, making the calcium
channel subunits target for therapeutic interventions (Burgess and
Noebels, 1999).
The 2 family consists of three genes. The
first subunit identified was 2-1 in rabbit
skeletal muscle (Ellis et al., 1988). Five tissue-specific splice
variants exist (Angelotti and Hofmann, 1996), but a functional
significance of the splicing has not been established. Two new
2 family members were subsequently
identified in human and mouse, and were named
2-2 and -3 (Klugbauer et al., 1999). The
novel 2 subunits are 56 and 30% homologous
to 2-1 at the amino acid level and share a
number of structural motifs. The subunits have similar hydrophobicity
profiles and all contain several potential N-glycosylation
sites. Northern analysis has shown that 2-1
is ubiquitously expressed, 2-2 is found in
several tissues including brain and heart, and
2-3 is brain-specific (Klugbauer et al.,
1999). An association of 2-2 with tumors
has been suggested, and the mouse homolog is a candidate for the
ducky epileptic phenotype (Gao et al., 2000).
2-1 consists of two proteinsa highly
glycosylated 2 that is believed to be
extracellularly located, and a smaller protein that anchors the
2 to the cell membrane (Brickley et al., 1995; Wiser et al., 1996). These proteins are coded for by a single gene, the
product of which is translated as a precursor polypeptide that is
post-translationally cleaved (De Jongh et al., 1990). The
2 and associate by disulfide bridges that
form between the numerous cysteine residues found in both proteins.
The effects of 2-1on the biophysical
properties of 1 subunits depend on the
expression system and subunits used. The subunit invariably increases
the current density of calcium channels by increasing the amount of
functional channel at the cell surface, and has been reported to
allosterically alter the activation and inactivation of several
1 subunits (Singer et al., 1991; Bangalore et
al., 1996, Felix et al., 1997, Klugbauer et al., 1999).
2-1 is known to enhance dihydropyridine
binding to L-type channels and 
-conotoxin GVIA to N-type channels
(Brust et al., 1993; Felix et al., 1997).
2-2 and -3 significantly enhance and
modulate the current through a number of HVA and LVA channels
(Klugbauer et al., 1999; Gao et al.; 2000, Hobom et al., 2000). The
action of these subunits depends on the 1
subunit expressed and 2-2 and -3 may
preferentially interact with Cav2.3
(1E), Cav2.1
(1A), or even Cav3.1
(1G).
Gabapentin (GBP) is an antiepileptic drug that has also found
application in pain and anxiolytic disorders (Welty et al., 1993;
Beydoun et al., 1995). GBP binds to rat brain (Hill et al., 1993) and
skeletal muscle homogenates (Gee et al., 1996), with lower binding seen
in heart, lung, and pancreas (Suman-Chauhan et al., 1993). GBP was
subsequently found to bind specifically to
2-1 of voltage activated calcium channels
(Gee et al., 1996). Because voltage activated channels are involved in
controlling the electrical excitability of neurons, it has been
postulated that this drug reduces calcium current by modulating
1 indirectly through its association with
2-1 (Gee et al., 1996).
The purpose of this study was to characterize the gross structure and
properties of the novel 2-2 and -3 subunits. It was found that 2-1, -2, and -3 are similarly processed and post-translationally modified.
2-1 and -2 bound GBP with differing
affinities, but the more distantly related
2-3 did not.
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Materials and Methods |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Transfection of COS-7 Cells.
Plasmids containing the
2 subunits, or pcDNA3 (Invitrogen,
Groningen, The Netherlands) as control, were transiently transfected in
COS-7 cells, using FuGene 6 (Roche, Mannheim, Germany).
2-1 and -3 had been previously cloned into
the expression vector pcDNA3, and 2-2 into
pcDNA3.1/V5/His-TOPO (Klugbauer et al., 1999). The cells were
maintained in Dulbecco's modified Eagle's medium (Life Technologies,
Karlsruhe, Germany) containing 10% fetal calf serum, 100 U of
penicillin, and 100 µg/ml streptomycin at 37°C, 6%
CO2; the cells were seeded at 1.5 × 106 cells per 100-mm culture plate. After 24 h, the cells were transfected in antibiotic-free medium with 6 µg of
DNA using 18 µl of FuGene reagent per plate. The medium was replaced
with complete medium after 16 h and harvested 60 to 72 h
after the start of transfection.
Membrane Preparations.
Tissues from BALB/c mice were crushed
under liquid nitrogen using a mortar and pestle. The powder was
homogenized in buffer A (20 mM MOPS, pH 7.4, 300 mM sucrose, 2 mM EDTA,
1 mM iodoacetamide, 1 mM orthophenanthroline, 0.2 mM
phenylmethylsulfonyl fluoride, 1 mM benzamidine, 1 µg/ml
leupeptin, 1 µg/ml pepstatin A, and 1 µg/ml antipain) by two 20-s
bursts with a Polytron homogenizer (Kinematica AG, Switzerland) and 8 strokes in a power-driven Potter pestle (Braun Biotech,
Germany). Cell debris was pelleted by centrifugation at
5000 g for 10 min at 4°C. Low-speed pellets were re-extracted as
above and the supernatants combined. The supernatants were centrifuged
at 70,000 g for 30 min at 4°C. The pellets were resuspended in buffer
A and stored in aliquots at 
80°C. Membranes from transfected COS-7
cells were prepared similarly, with the following modifications: cells
were harvested by scraping into 1× phosphate-buffered saline, pelleted
by low speed centrifugation, resuspended in 5 mM Tris-Cl, 5 mM EDTA, pH
7.4, containing protease inhibitors (as above) and incubated on ice for
15 min before homogenization. The pellets resulting from
ultracentrifugation were resuspended in 50 mM MOPS, pH 7.4, plus
protease inhibitors. The protein content was determined by the Bradford
method using BSA as a standard.
Anti-Peptide Antibodies.
Antibodies were raised in rabbits
by Gramsch Laboratories (Schwabhausen, Germany) against peptides of the
human 2-2 (amino acids 98-115) and murine
2-3 (amino acids 59-76) subunits
(Klugbauer et al., 1999). These sequences were selected because they
have low homology to each other and to 2-1,
are found after the putative signal peptide sequence, and have no
potential N-glycosylation sites. The antibodies were
affinity purified using a SulfoLink coupling gel (Pierce, Rockford, IL)
with bound antigen. Antibodies were eluted with 4.5 M
MgCl2, and concentrated using Centricon YM-50
centrifugal filter devices (Millipore Corporation, Bedford, MA). The
antibody was made to 1 mg/ml BSA in phosphate-buffered saline and
stored at 20°C in aliquots.
Western Blotting.
Proteins were separated by discontinuous
SDS-PAGE in 5 or 7.5% resolving gels. The membrane preparations were
denatured in Laemmli sample buffer (with or without 0.1 M
dithiothreitol) by boiling for 3 min. Typically, 50 to 100 µg of
tissue or 3 µg of COS-7 microsomal membrane preparation was loaded
per lane. After electroblotting and blocking in 3% BSA, the
nitrocellulose membranes were incubated for 2 h at room
temperature with primary antibodies used at 1/750 for
2-2 and 1/500 for
2-3. A commercially available anti-2-1 monoclonal antibody (ABR, Golden,
CO) was used at a concentration of 1/500. Incubation with the secondary
goat anti-rabbit- or goat anti-mouse-horseradish peroxidase antibodies
(Dianova, Germany) proceeded for 1 h at room temperature at a
dilution of 1/7000. Antibody binding was detected using the ECL system
(Amersham Pharmacia Biotech, Freiburg, Germany).
Deglycosylation Assay.
Membrane protein (70 µg) was
denatured by boiling in 0.1 M -mercaptoethanol, 0.5% SDS for 5 min.
The reaction was brought to 15 mM Tris-Cl, pH 8.0, 20 mM
orthophenanthroline, and 1% Triton X-100. Two units of
N-glycosidase F (Roche, Mannheim, Germany) were added and
the reaction allowed to proceed for 5 h at 37°C. The protein was
separated by SDS-PAGE gel and analyzed by Western blotting as described above.
Gabapentin Binding Assay. COS-7 membrane preparations (10 to 30 µg) were incubated in 200 µl volumes with various concentrations of [3H]gabapentin (143 Ci/mmol, custom synthesized by Amersham Pharmacia Biotech, Little Chalfont, Buckinghamshire, UK) in 10 mM HEPES/KOH, pH 7.4, for 30 min at room temperature. The protein was precipitated using 8 ml of ice-cold precipitation buffer (22.5 mM HEPES, pH 7.4; 11.25% polyethylene glycol 6000; 11.25 mM CaCl2) and filtered over GF/B filters soaked in the same buffer. Two further 8-ml volumes of precipitation buffer were used as washes. The activity of the filters was counted in a scintillation counter. Concentrations greater than 20 nM were achieved by adding nonradioactive gabapentin to the required concentration. The corrected binding was calculated using the equation, Total GBP bound = (specific dpm) × [1 + (concentration nonradioactive gabapentin/concentration [3H]gabapentin)].
Nonspecific binding was determined in the presence of 10 µM unlabeled gabapentin. The background binding was less than 20% of the counts without addition of unlabeled gabapentin. To assess the effect of the carbohydrates on GBP binding, 30 µg of native mouse brain membranes were incubated with 2 U of N-glycosidase F in 15 mM Tris-Cl containing protease inhibitors (as used for preparation of the membranes), for 18 h at 37°C without prior denaturing.| |
Results |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Analysis of 2 Protein Structure.
The
specificity of the peptide antibodies was tested using membrane
preparations of COS-7 cells transfected with the various 2 proteins. The commercial
2-1 antibody did not recognize 2-2 and -3 preparations. Similarly, the
peptide antibodies only recognized the 2
against which they were raised (Fig. 1).
The antibodies were also preincubated with an excess of peptide antigen before incubation with the protein blots to test for cross-reactivity. The bands corresponding to the 2 proteins
were not detected, indicating that the antibodies are specific (results
not shown).
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2
proteins, various murine tissues were analyzed by Western blotting. In
our study, 2-1 in brain had a mass of 200 kDa under nonreducing conditions and 140 kDa in a reducing environment
(Fig. 2), which is in accord with the
values reported previously (Jay et al., 1991).
2-2 in mouse brain had an apparent
molecular mass of 190 kDa under nonreducing conditions, which shifted
to 138 kDa when DTT was added. 2-3 in brain
had the lowest mobility of the 2 proteins, with a mass of 166 kDa under nonreducing and 131 kDa under reducing conditions (Fig. 2A). Our results indicate that, similar to
2-1, 2-2, and
2-3 consist of separate, disulfide linked
2 and proteins. Because the antibodies
recognize the amino-terminal domains of the
2-2 and -3 subunits, which correspond to
the putative 2, the shift in migration is due
to the loss of the protein caused by reduction of the disulfide
bonds. The mass estimated by subtraction for of
2-1 is 53 kDa, 57 kDa for 2-2, and 35 kDa for
2-3. A shift in electrophoretic mobility of
both 2-2 and -3 upon reduction was also
observed in COS-7 membranes expressing the proteins (Fig. 4, insert).
The multiple bands detected are most probably caused by the
glycosylation and processing of the overexpressed proteins by the COS-7
cells.
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2 proteins (Fig. 2B).
The tissue distribution of the three 2
subunits in mouse was also analyzed by immunoblotting. As can be seen
in Fig. 3, 2-1 is expressed in all tissues studied,
namely brain, heart, skeletal muscle, liver, and lung. The highest
expression was seen in skeletal muscle and brain; in the latter case
only 40 µg of protein was used while 100 µg of the other
preparations were loaded. The heart subunit had a larger apparent mass
than that of the brain subunit 150 kDa as compared with 140 kDa
(reducing conditions). The 2-1b splice
variant is exclusively found in brain, whereas the predominant forms in
heart are 2-1c and -d (Angelotti and Hofmann, 1996). Because the 2-1c and -d
heart splice variants have 5 and 12 fewer amino acids than that of the
brain isoform, respectively, the difference in mass is believed to be
caused by glycosylation.
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2-2 was found to be expressed at high
levels in brain and, to a lesser extent, in heart (Fig. 3). Weaker
reactive bands of a similar size were seen in lung, liver, and skeletal
muscle, in addition to bands at approximately 120 kDa in brain, heart, and lung. The apparent mass of the primary reactive band in heart was
153 kDa under reducing conditions, which is larger than that seen for
2-2 in brain (138 kDa). This may also be
caused by differential glycosylation and/or splice variation, because
four splice variants have been described so far for
2-2 (Gao et al., 2000; Hobom et al., 2000).
To determine whether the protein detected in the tissues is in fact
2-2, the antibody was preincubated with an
excess of antigen. The bands at approximately 160 and 120 kDa
disappeared, indicating a specific reaction (data not shown). Because
the antibody recognized both bands, the protein detected at lower
masses is caused by the presence of more than one splice form,
partial degradation, or incompletely processed forms of the highly
glycosylated protein. The latter option is possible as the membrane
preparations also contain endoplasmic reticulum with associated
protein. 2-3 was only found to be expressed
in brain, and the smears below and above the size expected for
2-3 in skeletal muscle are believed to be
caused by spurious reactions with contractile elements (Fig. 3).
Gabapentin Binding Assays.
Binding of GBP to the
2 subunits was assessed using COS-7 cells
that overexpressed the proteins. Membrane preparations were incubated
with [3H]gabapentin for 30 min. The protein was
subsequently precipitated, captured on filters, and measured by
scintillation counting. 2-1 and
2-2 were found to specifically bind GBP,
whereas 2-3 did not show any binding (Fig.
4). Cells transfected with pcDNA3 alone as a control did not interact with GBP. 2-1
bound GBP with a relatively high affinity, and a dissociation constant
(Kd) of 59 ± 6 nM (S.E.M.) was
calculated by Scatchard analysis of data from three experiments (Fig.
5). 2-2 was
found to bind GBP with a Kd of 153 ±14 nM
(S.E.M.) in six independent experiments. In both cases, GBP seemed to
bind to a single binding site, as judged by the Scatchard plots. The
contribution of 2 carbohydrate side chains
to GBP binding was also investigated. The binding of
[3H]GBP to native mouse brain membranes
following deglycosylation for 18 h with N-glycosidase F
was not significantly altered relative to controls incubated without
enzyme (not shown).
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Discussion |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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This study was undertaken to clarify the gross protein structure
and characteristics of the novel 2-2 and -3 subunits. It was of particular interest to determine whether the
characteristic traits of 2-1, namely its
composition of two proteins derived from a single precursor protein,
and its high level of glycosylation, are conserved. Because GBP, a drug
increasingly used for neurological disorders, binds to
2-1, the novel subunits were also tested for drug binding.
Using antibodies directed against the putative
2 of the 2-2 and
-3 subunits, it could be assessed whether precursor proteins are
cleaved and form complexes via disulfide bridges. Both
2-2 and -3 in native tissues were found to
be composed of an 2 and , which could be
separated by reduction. The difference in mass of the nonreduced
complex relative to the reduced protein roughly corresponds to that of
alone and was approximately 50 kDa for each of the
2 proteins. The cleavage site of
2-1 is between A934
and A935, when the signal sequence is not taken
as part of the protein (De Jongh et al., 1990; Jay et al., 1991). The
alanine at position 934 in 2-1 is conserved
in 2-2 and -3, although the rest of the
sequence in the region diverges. Although the
2-1 cleavage site cannot be assumed to be
the same as for the novel proteins, the approximate sizes of the proteins and the conservation of the alanine suggest that this could be
the case. If the alanine is assumed to be the first residue of for
both 2-2 and -3, then the mass calculated
for of 2-2 based on its amino acid content is 17.2 kDa, and for 2-3, 15.1 kDa.
The mass estimated indirectly is larger than that calculated using the
amino acid sequence. This difference is likely to be due to the
difficulty associated with inferring sizes based on shifts in SDS-PAGE
migration of reduced and nonreduced proteins, as well as
post-translational modifications such as N-glycosylation
(both proteins contain potential N-glycosylation sites).
A similar pattern of modification has been observed for the of
2-1, which has a calculated mass of 19 kDa,
and a migration of 24 and 27 kDa using antibodies against the (De
Jongh et al., 1990).
All three 2 proteins were found to be
highly glycosylated, with 30 kDa of the mass of the proteins consisting
of oligosaccharides. Because glycosylation is essential for current
stimulation by 2-1 of
Cav2.1 (1A) (Gurnett et
al., 1996), this is likely to be the case for the novel subunits as well.
The distribution of 2 protein in mouse
tissue was compared with that of the mRNA expression pattern (Klugbauer
et al., 1999). 2-3 was detected only in
brain, which corresponds with the results of the Northern analysis.
2-2 mRNA was originally described to be
ubiquitously expressed, with the highest levels in brain, heart,
pancreas, and skeletal muscle (Klugbauer et al., 1999). Lower levels of
the mRNA were seen in other tissues after longer exposures. In this
study, 2-2 protein was detected at very low levels in skeletal muscle, although the Northern analysis had produced
a signal comparable with brain. Gao et al. (2000) reported high levels
of 2-2 mRNA in human lung and cloned the
subunit from a lung library. Although 2-2
protein was observed at low levels in mouse lung in this study, it is
possible that certain lung cell types express high levels. Whereas the
Gao group showed overexpression of 2-2
protein in various tumor cell lines, no data was presented on the
endogenous levels in healthy lung tissue.
The specific binding of gabapentin to 2-1
was the first described interaction between a regulatory subunit of
voltage activated calcium channels and a pharmaceutical agent. The
Kd of porcine brain
2-1 was reported as 9.4 nM (Brown et
al., 1998) but as 37.5 nM for porcine
2-1 expressed in COS-7 cells (Brown and Gee, 1998) and 16 nM for rabbit 2-1 in
COS-7 cells (Gee et al., 1996). In this study,
Kd values of 59 nM for
2-1 and 153 nM for
2-2 were determined. In a preliminary
report by Su et al. (2000), 2-2 is
described as having two binding sites (Kd
values of 147 and 25 nM). The reason for variations in
Kd values is not clear, but may be
attributable to species differences and assay methods. Because GBP is
used for a variety of neurological disorders, it is interesting to note
that it binds to two auxiliary calcium channel subunits that have been
found to exert differing modulatory effects on
1 pore subunits in heterologous expression systems.
The effect of GBP on the physiological activity of calcium channels is
not clearly understood. In patch-clamp studies with hippocampal granule
cells, no effect of GBP was reported (Schumacher et al., 1998).
However, in other studies, modest to dramatic changes in calcium
current were noted. A reduction in the calcium current in isolated
neurons (Stefani et al., 1998) and in rat neocortical slices (Fink et
al., 2000) upon application of GBP has been described. Calabresi et al.
(2000) found GBP to reduce most excitatory properties of striatal spiny
neurons, which could account for the anticonvulsant effect of the drug.
Dooley et al. (2000) have also shown that GBP and a related compound,
pregabalin, reduce the release of norepinephrine when stimulated by
potassium and electrical pulses. The calcium channels affected are not
known, but candidates are L-type (Stefani et al., 1998) and P/Q (Fink
et al., 2000; Meder and Dooley, 2000). No consistent effect of GBP on
Cav1.2 (1C), Cav2.1 (1A), and
Cav3.2 (1G) currents in
the heterologous human embryonic kidney 293 expression system were
observed in this study. The complexity of the interaction between GBP
and 2 is further illustrated by a
temperature dependent influence of ruthenium red,
MgCl2, and spermine on GBP binding (Taylor and
Bonhaus, 2000). Initial studies on GBP binding using rat tissue
homogenates showed strong binding in skeletal muscle and brain, where
2-1 is most highly expressed (Gee et al.,
1996). A much lower binding of the drug was seen in liver and kidney,
which express considerable levels of the protein, as judged by Western
blotting. A possible explanation for these conflicting results is that
the binding of GBP to 2 is modulated by
other subunits (e.g., the 1 pore protein). It
is possible that the effects of GBP depend on the composition and
environment of the channel. The lack of clinical side effects of the
drug on skeletal muscle and other 2-1
expressing tissues supports this view (Beydoun et al., 1995). GBP has
also been shown to be an agonist of certain -aminobutyric
acidB receptors, and this has also been
postulated to be involved in the clinical action of the drug (Ng et
al., 2001).
Gabapentin binding is dependent on the presence of both and subunits, which do not have to be translated as a single precursor protein (Wang et al., 1999). Their interaction is important, however, because neither nor bind the drug when expressed alone (Wang et
al., 1999). Cleavage of the precursor protein is also not required for
binding (Brown and Gee, 1998). Mutation analysis of porcine 2-1 by Brown and Gee (1998) led to the
identification of a region (960-994) in -1, containing a zinc-like
finger, that is important for gabapentin binding. Another study
identified residues 206 to 222, 516 to 537, and 383 to 603 as essential
for binding (Wang et al., 1999). Because
2-2 has in this study been shown to bind gabapentin, it is instructive to compare the sequences identified as
putative binding sites in previous reports (Fig.
6). Mutations of charged amino acids in
2-1 was performed by Wang et al. (1999), and Arg217 found to be the most important. This
residue is found in 2-2, but not in
2-3, supporting its role in the binding of
GBP. It is, however, not clear whether these sites are essential for
the association of 2 with , or whether they
form a gabapentin-binding pocket.
|
Gabapentin analogs have been developed that bind to
2-1 with a higher affinity than gabapentin
and are effective in an animal model of epilepsy (Bryans et al., 1998).
Because 2 subunits may associate
preferentially with 1 subunits in the brain,
these drugs could have differing therapeutic actions if more than one of 2 family binds these drugs.
In summary, we present results indicating that
2-2 and -3 consist of two proteins, derived
from a single transcript, that are associated by disulfide bonds. Both
novel subunits are highly glycosylated.
2-2, but not
2-3, is capable of binding the antiepileptic drug GBP, which has a higher affinity for
2-1 than for
2-2. Further investigation into the
molecular action of GBP and its analogs on voltage gated calcium
channels should enable the fine-tuning of treatment of neurological disorders.
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Acknowledgments |
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We thank Lubica Lacinová for electrophysiological experiments and Susanne Kamp for technical assistance.
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Footnotes |
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Received November 11, 2000; Accepted February 9, 2001
This research was supported by the Deutsche Forschungs Gemeinschaft and the Fond der Chemischen Industrie.
Send reprint requests to: Dr. N. Klugbauer, Institut für Pharmakologie und Toxikologie der Technischen Universität München, Biedersteiner Strasse 29, 80802 München, Germany. E-mail: klugbauer{at}ipt.med.tu-muenchen.de
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Abbreviations |
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HVA, high voltage activated; LVA, low voltage activated; GBP, gabapentin; MOPS, 3-(N-morpholino)propanesulfonic acid; BSA, bovine serum albumin; PAGE, polyacrylamide gel electrophoresis; DTT, dithiothreitol.
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References |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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2 subunit.
FEBS Lett
397:
331-337[Medline].2/-subunit on ionic and gating current in transiently transfected HEK 293 cells.
Am J Physiol
270:
H1521-H15282 subunit of voltage-gated Ca2+ channels.
FEBS Lett
364:
129-133[Medline].2 Ca2+ channel subunit from porcine brain: development of a radioligand binding assay for 2 subunits using [3H]leucine.
Anal Biochem
255:
236-243[Medline].2 calcium channel subunit from porcine cerebral cortex.
J Biol Chem
273:
25458-254652 subunit of a calcium channel and their evaluation as anticonvulsant agents.
J Med Chem
41:
1838-1845[Medline].1 and 2 subunits of a DHP sensitive calcium channel.
Science (Wash DC)
241:
1661-16642 subunit.
J Neurosci
17:
6884-68912 auxiliary subunit gene (CACNA2D2).
J Biol Chem
275:
12237-122422 subunit of a calcium channel.
J Biol Chem
271:
5768-57762 subunit in current stimulation and subunit interaction.
Neuron
16:
431-440[Medline].2-2 subunit.
Eur J Neurosci
12:
1217-1226[Medline].2-subunit and the associated peptides.
J Biol Chem
266:
3287-32932 subunit.
J Neurosci
19:
684-691-Aminobutyric acid type B receptors with specific heterodimer composition and postsynaptic actions in hippocampal neurons are targets of anticonvulsant gabapentin action.
Mol Pharmacol
59:
144-1522-2 subunit of calcium channel: a novel gabapentin binding protein in brain. Society for Neuroscience 30th Annual Meeting, 2000 Nov 4-9, New Orleans, LA. Society for Neuroscience, Washington DC.2 for gabapentin binding.
Biochem J
342:
313-320.2/ subunit of voltage sensitive Ca2+ channels is a single transmembrane extracellular protein which is involved in regulated secretion.
FEBS Lett
379:
15-20[Medline].
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 H. E. D. J. ter Keurs and P. A. Boyden Calcium and Arrhythmogenesis Physiol Rev, April 1, 2007; 87(2): 457 - 506. [Abstract] [Full Text] [PDF]
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|
 S. Sonkusare, M. Fraer, J. D. Marsh, and N. J. Rusch Disrupting Calcium Channel Expression To Lower Blood Pressure: New Targeting of a Well-Known Channel Mol. Interv., December 1, 2006; 6(6): 304 - 310. [Abstract] [Full Text] [PDF]
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A. Davies, L. Douglas, J. Hendrich, J. Wratten, A. Tran Van Minh, I. Foucault, D. Koch, W. S. Pratt, H. R. Saibil, and A. C. Dolphin The Calcium Channel {alpha}2{delta}-2 Subunit Partitions with CaV2.1 into Lipid Rafts in Cerebellum: Implications for Localization and Function. J. Neurosci., August 23, 2006; 26(34): 8748 - 8757. [Abstract] [Full Text] [PDF]
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H. Khosravani and G. W. Zamponi Voltage-gated calcium channels and idiopathic generalized epilepsies. Physiol Rev, July 1, 2006; 86(3): 941 - 966. [Abstract] [Full Text] [PDF]
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 S.-S. Choi, Y.-C. Kim, Y. J. Lim, C.-J. Lee, P.-B. Lee, S.-C. Lee, W.-S. Sim, and Y.-L. Choi The Neurological Safety of Epidural Gabapentin in Rats: A Light Microscopic Examination Anesth. Analg., November 1, 2005; 101(5): 1422 - 1426. [Abstract] [Full Text] [PDF]
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|
 C. Canti, M. Nieto-Rostro, I. Foucault, F. Heblich, J. Wratten, M. W. Richards, J. Hendrich, L. Douglas, K. M. Page, A. Davies, et al. The metal-ion-dependent adhesion site in the Von Willebrand factor-A domain of {alpha}2{delta} subunits is key to trafficking voltage-gated Ca2+ channels PNAS, August 9, 2005; 102(32): 11230 - 11235. [Abstract] [Full Text] [PDF]
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 M. O. Urban, K. Ren, K. T. Park, B. Campbell, N. Anker, B. Stearns, J. Aiyar, M. Belley, C. Cohen, and L. Bristow Comparison of the Antinociceptive Profiles of Gabapentin and 3-Methylgabapentin in Rat Models of Acute and Persistent Pain: Implications for Mechanism of Action J. Pharmacol. Exp. Ther., June 1, 2005; 313(3): 1209 - 1216. [Abstract] [Full Text] [PDF]
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K. C. Cundy, T. Annamalai, L. Bu, J. De Vera, J. Estrela, W. Luo, P. Shirsat, A. Torneros, F. Yao, J. Zou, et al. XP13512 [({+/-})-1-([({alpha}-Isobutanoyloxyethoxy)carbonyl] aminomethyl)-1-cyclohexane Acetic Acid], A Novel Gabapentin Prodrug: II. Improved Oral Bioavailability, Dose Proportionality, and Colonic Absorption Compared with Gabapentin in Rats and Monkeys J. Pharmacol. Exp. Ther., October 1, 2004; 311(1): 324 - 333. [Abstract] [Full Text] [PDF]
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C.-Y. Li, Y.-H. Song, E. S. Higuera, and Z. D. Luo Spinal Dorsal Horn Calcium Channel {alpha}2{delta}-1 Subunit Upregulation Contributes to Peripheral Nerve Injury-Induced Tactile Allodynia J. Neurosci., September 29, 2004; 24(39): 8494 - 8499. [Abstract] [Full Text] [PDF]
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 S. V. Ivanov, J. M. Ward, L. Tessarollo, D. McAreavey, V. Sachdev, L. Fananapazir, M. K. Banks, N. Morris, D. Djurickovic, D. E. Devor-Henneman, et al. Cerebellar Ataxia, Seizures, Premature Death, and Cardiac Abnormalities in Mice with Targeted Disruption of the Cacna2d2 Gene Am. J. Pathol., September 1, 2004; 165(3): 1007 - 1018. [Abstract] [Full Text] [PDF]
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 J. Brill, R. Klocke, D. Paul, D. Boison, N. Gouder, N. Klugbauer, F. Hofmann, C.-M. Becker, and K. Becker entla, a Novel Epileptic and Ataxic Cacna2d2 Mutant of the Mouse J. Biol. Chem., February 20, 2004; 279(8): 7322 - 7330. [Abstract] [Full Text] [PDF]
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Z. D. Luo, N. A. Calcutt, E. S. Higuera, C. R. Valder, Y.-H. Song, C. I. Svensson, and R. R. Myers Injury Type-Specific Calcium Channel alpha 2delta -1 Subunit Up-Regulation in Rat Neuropathic Pain Models Correlates with Antiallodynic Effects of Gabapentin J. Pharmacol. Exp. Ther., December 1, 2002; 303(3): 1199 - 1205. [Abstract] [Full Text] [PDF]
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 N. Qin, S. Yagel, M.-L. Momplaisir, E. E. Codd, and M. R. D'Andrea Molecular Cloning and Characterization of the Human Voltage-Gated Calcium Channel alpha 2delta -4 Subunit Mol. Pharmacol., September 1, 2002; 62(3): 485 - 496. [Abstract] [Full Text] [PDF]
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A. A. Jensen, J. Mosbacher, S. Elg, K. Lingenhoehl, T. Lohmann, T. N. Johansen, B. Abrahamsen, J. P. Mattsson, A. Lehmann, B. Bettler, et al. The Anticonvulsant Gabapentin (Neurontin) Does Not Act through gamma -Aminobutyric Acid-B Receptors Mol. Pharmacol., June 1, 2002; 61(6): 1377 - 1384. [Abstract] [Full Text] [PDF]
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