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J. Biol. Chem., Vol. 277, Issue 23, 20678-20685, June 7, 2002
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From the
Received for publication, January 23, 2002, and in revised form, March 14, 2002
Eye tissues contain splice variants of
muscle-preferred p94 (calpain 3), such as lens-specific Lp82 and Lp85,
retina-specific Rt88, and cornea-specific Cn94. The purpose of the
present experiment was to analyze the activation and regulation of the
best characterized p94 splice variant, Lp82. Recombinant rat Lp82
(rLp82) was expressed using the baculovirus system, purified with
Ni-NTA affinity and DEAE-ion exchange chromatographies, and
characterized by SDS-PAGE, casein zymography, and immunoblotting. After
incubation with calcium, rLp82 autolyzed into two major fragments at
~60 and 22 kDa. Sequencing of the autolytic fragments showed loss of
three amino acids from the N terminus and cleavage near the IS2 region.
Also, Lp82 and calpain 2 were found to hydrolyze each other.
Calpastatin inhibited calpain 2 activity, but not Lp82. Homology
modeling suggested that the lack of inhibition of Lp82 by
calpastatin was due to molecular clashes at the unique AX1 region of
Lp82. Lp82 also hydrolyzed calpastatin. These results suggested that
Lp82 might regulate other calpain activities and cause hydrolysis of
substrates such as crystallins during lens cataract formation.
Calpains (EC 3.4.22.17) comprise a family of non-lysosomal,
cysteine proteases with a neutral pH optimum and a requirement for
calcium for activation (1). They are widely distributed in animal
tissues, where they are involved in a variety of cellular processes
involving calcium (2). Calpains consist of the ubiquitous calpains 1 (µ-calpain), 2 (m-calpain), and 10; and tissue-specific calpains such
as 3 (muscle-specific p94), 8, and 9 (3-6). Recently, splice variants
of calpain 3 such as lens-specific Lp82 and Lp85, retina-specific Rt88,
and cornea-specific Cn94 were found in the eye (7-10). Tissue-specific
calpains may have unique properties or structures distinct from the
ubiquitous calpains. For example, mutations in muscle-preferred p94
calpain cause muscular dystrophy type 2A in man (11). p94 contains
three unique regions: the novel N-terminal sequence
(NS),1 insert region 1 (IS1),
and insert region 2 (IS2) (4).
Lens-specific calpain Lp82 belongs to a new subclass of calpains,
termed AX1, because they replace the NS region in the N-terminal domain
I by using alternative exon 1, a
portion of the 3' end of intron 1 from the p94 gene. Common promoter
elements in the eye may cause the alternative transcription of AX1 from
the p94 gene. Other p94 variants contain combinations of splice
variations in or near the IS1 and IS2 insert regions. Lp82 activity in
young rat lenses is abundant and stable, because the IS1 and IS2
regions are splice deleted (12, 13). Besides Lp82, rodent lenses
contain ubiquitous calpain 2, atypical and ubiquitous calpain 10, and lens-specific Lp85. These calpains may regulate each other by proteolysis, because they are substrates for each other. Thus, the
purpose of the present experiment was to study calpain interactions by
analyzing the activation and regulation of Lp82 in lens.
Animals--
Experiments were performed using male
Sprague-Dawley rats at 12 days of age. Experimental animals were
handled in accordance with The Association for Research in Vision and
Ophthalmology Statement for the Use of Animals in Ophthalmic and
Vision Research and the Guiding Principles in the Care and Use of
Animals (Department of Health, Education, and Welfare
Publication, NIH 80-23).
Expression of Recombinant Lp82 Using the Baculovirus
System--
The cDNA for Lp82 from rat was cloned into a pFASTBAC
HTb vector (Invitrogen) containing a His tag and rTEV protease cleavage site in the N terminus. This plasmid was transformed into
DH10BAC-competent cells (Invitrogen), which contain the bacmid and the
helper plasmid. Recombinant bacmid DNA containing Lp82 cDNA was
isolated and used to transfect Spodoptera frugiperda 9 (Sf9) insect cells. Transfection was performed with recombinant
Lp82 (rLp82) baculovirus amplified to 108 plaque-forming
units/ml. Sf9 cells were cultured for 3 days for rLp82 protein expression.
Purification of rLp82--
Cultured cells were sonicated in
lysis buffer containing 20 mM Tris (pH 7.5), 0.5 mM EGTA, and 2 mM dithioerythritol. The soluble protein was obtained by centrifugation at 13,000 × g for 30 min. Soluble Lp82 was purified by Ni-NTA (Qiagen
Inc, Valencia, CA) metal-affinity chromatography according to the
manufacturer's protocol under native conditions. Further purification
was performed by high performance liquid chromatography using a
7.5-mm inner diameter × 7.5-cm DEAE 5PW column (TOSOH, Japan)
with a linear 0.0-0.5 M NaCl gradient in buffer A
containing 20 mM Tris (pH 7.5), 1 mM EDTA, 1 mM EGTA, and 2 mM dithioerythritol at 1 ml min Activation of rLp82--
Purified rLp82 was incubated with 1.4 mM calcium in 20 mM Tris buffer (pH 7.5) for
10, 20, 30, 40, 50, 60, and 90 min.
Hydrolysis of Calpains by Other Calpains--
To inactivate
calpains, purified rLp82 and recombinant calpain 2 (rcalpain 2) from
rat (more than 98% purity, Calbiochem) were incubated with 5 mM iodoacetamide in 20 mM Tris buffer (pH 7.5)
at 37 °C for 2 h. After quenching excess iodoacetamide with 10 mM dithioerythritol, 1.2 units of rcalpain 2 or
rLp82 were added and incubated with calcium for 1 h at 37 °C.
Fragments were detected by SDS-PAGE and immunoblotting.
Sensitivity of Calpains to Inhibition by Calpastatin--
0.22
units of rcalpain 2 or rLp82 were incubated for 1 h at 37 °C
with 0.5 µM calpastatin purified from human erythrocytes (Calbiochem) and 1.5 mM calcium. Hydrolyzed calpastatin
fragments were detected by SDS-PAGE. Immunoblotting and casein
zymography were used to detect calpain degradation and calpain
activity, respectively.
Electrophoresis and Immunoblotting--
SDS-PAGE was performed
on discontinuous, 8 or 12% gels (Invitrogen) using the glycine buffer
system. Immunoblots for Lp82 and calpain 2 were performed by
electrotransferring proteins from SDS-PAGE gels to polyvinylidene
difluoride membrane at 30 V (constant) for 100 min at an ice-cold
temperature using Tris-glycine buffer (12 mM Tris, 96 mM glycine, 20% methanol). The anti-Lp82 antibody and
anti-calpain 2 antibodies were used at 1:1000 dilution, and immunoreactivity was visualized with 5-bromo-4-chloro-3-indolyl phosphate/nitro blue tetrazolium and alkaline phosphatase conjugated to
anti-rabbit IgG secondary antibody (Bio-Rad).
Casein Zymography--
8% (1-mm thick) gels, co-polymerized
with 0.05% casein were pre-run with a buffer containing 25 mM Tris (pH 8.3), 192 mM glycine, 1 mM EGTA, and 1 mM dithiothreitol for 15 min at
4 °C. Samples were then loaded and run. After electrophoresis, the
gels were incubated with slow shaking overnight at room temperature in
20 mM Tris (pH 7.4), 10 mM dithiothreitol, and
2 mM calcium. Gels were stained with Coomassie Brilliant
Blue. Bands of caseinolysis appeared white.
N-terminal Sequencing of Autolytic Fragments--
rLp82 was
autolyzed by incubating in 1.4 mM calcium for 10 and 90 min
at 30 °C, and 12% SDS-PAGE (1 mm thick) gels were then run and
transferred onto polyvinylidene difluoride membrane at 30 V (constant)
for 100 min. Membranes were stained with 0.1% Coomassie Brilliant Blue
in 50% methanol for 10 min and destained with 50% methanol. Destained
membranes were dried, and bands were excised for Edman N-terminal
sequencing. Proteins (or peptides) were sequenced by Deb McMillen in
the Biotechnology Laboratory at the University of Oregon, Eugene, OR,
on an Applied Biosystems model 492 Procise N-terminal protein sequencer
using N-terminal Edman degradation chemistry.
Phenylthiohydantoin-derivatives were identified with an Applied
Biosytems model 140 PTH Analyzer and a model 785A detector set at
wavelength 269 nm.
Homology Modeling of Lp82 and Calpain 3--
Protein homology
modeling was performed on a Silicon Graphics OCTANE2 work station,
using MOE (The Molecular Operating Environment, Version 2001.01, Chemical Computing Group Inc., Montreal, Canada, www.chemcomp.com).
The Brookhaven Protein Data Bank (14) was used as the structural
template for building homology models. The rat Lp82 and rat calpain 3 sequences were taken from the NCBI Protein Data Base (NCB accession
numbers AAC04848 and AAA41790, respectively). Each sequence was aligned
to the template sequence (human calpain 2, Protein Data Bank number
1KFU) using the protein alignment tools in MOE. The alignment
conditions were tree-based using an initial pair-wise buildup followed
by round robin and iterative refinement. The group-to-group calculation used the Gonnet substitution matrix and had a gap start penalty of 3 and a gap extend penalty of 1. The alignment was not biased by either
actual or predicted secondary structure.
The homology modeling procedure involved building three-dimensional
models of both sequences using human calpain 2 as a template structure.
Two types of models were considered. The first assumed that Lp82
co-existed with calpain 4, thus all atoms of calpain 4 were included
during the modeling and minimization. The other type of model did not
consider calpain 4 as part of the final structure. In addition, models
were constructed so that the outgap residues (residues that extend
beyond the terminals of the template chain) were either ignored or
included in the modeling procedure. Homology modeling generated ten
intermediate models, from which the best scoring model was chosen and
minimized to produce the final model (Amber89 forcefield, root mean
square distance = 0.01).
To investigate the potential interaction of Lp82 with calpain 4, van
der Waals (VDW) interaction energies were calculated and are reported
on Fig. 7. The structure labeled Lp82* was constructed with
the assumption that calpain 4 was present, with the outgap residues
included. Calpain 3 models did not include the presence of calpain 4, since calpain 3 is well known not to associate with calpain 4 (16).
Autolysis of Lp82--
To test if Lp82 is autolytic, rLp82 was
incubated with calcium for 0-90 min. Unautolyzed, intact rLp82
migrated at 85 kDa instead of 82 kDa (Fig.
1, lane marked "0 min").
This is because rLp82 contains 26 additional amino acids in the N
terminus from the His tag and vector protease cleavage site. Autolytic
fragments at 82, 60, and 22 kDa appeared after incubation with calcium
(Fig. 1A, arrows). Production of these fragments
was inhibited by addition of EGTA or cysteine protease inhibitor E64
(data not shown).
The origin of the fragments from Lp82 autolysis was determined by
immunoblotting using two different antibodies. One antibody recognized
epitopes near the deleted IS2 region at the end of Lp82 domain III
(Fig. 1B, lanes 1-3), while the second antibody recognized the N terminus (Fig. 1B, lanes 4-6).
The 82-kDa autolytic fragment reacted with both antibodies, the 60-kDa
fragment reacted only with the N-terminal antibody, and 22 kDa was
visualized only with the IS2 antibody. These results suggested that the
82- and 60-kDa fragments contained the N-terminal region, while the
22-kDa fragment was the C-terminal region. This was confirmed by direct N-terminal sequencing of the 82- and 22-kDa fragments (Fig.
2). The 82-kDa fragment showed loss of 29 amino acids from the N terminus. This included 3 amino acids from Lp82,
the His tag region, and the protease cleavage site domain from the
vector (Fig. 2A). The autolytic cleavage producing the new
N-terminal sequence on the 22-kDa fragment started at arginine
(R) residue 524 near the deleted IS2 region (Fig.
2B). The location of autolytic sites in intact Lp82 is
showed in Fig. 2C. Thus, the 82-kDa fragment was
rLp82-truncated at leucine 30 in the N terminus, the 60-kDa fragment
was comprised of residues from leucine (L) 30 to aspartic
acid (D) 549, and the 22 kDa was from arginine
(R) 550 near the IS2 region to the C-terminal alanine
residue (A) 735.
Interaction between calpains--
Since rodent lenses contain
calpain 2 and calpastatin in addition to Lp82, we next investigated how
these components of the calpain system interacted with each other. This
was accomplished by inactivating rcalpain 2 and rLp82 by alkylation of
the active site cysteine and then testing to see whether the
proteins were proteolyzed by fresh, active rLp82 or rcalpain 2 (Fig.
3) as detected by SDS-PAGE (Fig.
3A), and immunoblotting with Lp82 (Fig. 3B) and
calpain 2 antibodies (Fig. 3C). When active Lp82 was
incubated with inactive calpain 2 protein in the presence of calcium,
the calpain 2 protein at 80 kDa was decreased (lane 5 in
Fig. 3, A-C). When calcium was omitted, Lp82 and calpain 2 were not degraded (lane 4). Of course, addition of active
Lp82 to inactive Lp82 protein caused a decrease in the Lp82 band
(lane 6), and this was a confirmation of autolysis described
above. In the converse experiment, when active calpain 2 was added to
inactive Lp82 substrate, Lp82 was totally hydrolyzed (lane
2). Calpain 2 also autolyzed itself (lane 3). Thus,
Lp82 and calpain 2 hydrolyzed each other, although Lp82 seemed the more
sensitive substrate for calpain 2.
Hydrolysis of Calpastatin--
Calpastatin (CS) purified from
human erythrocytes migrated to 65 kDa on SDS-PAGE (Fig.
4A, lane 1).
Incubation of this CS with calpain 2 activated by calcium did not cause
breakdown of CS (Fig. 4A, lane 2). Immunoblotting
revealed that the calpain 2 did not undergo autolysis when it was
incubated with CS (Fig. 4B, lane 2), and the CS
completely inhibited calpain 2 activity (Fig. 4C, lane
2). Thus, CS was not a substrate for calpain 2, because CS
inhibited calpain 2. In contrast, incubation of calcium-activated Lp82
with CS caused total hydrolysis of CS (Fig. 4A, lane
4). This was accompanied by a decrease in apparent molecular mass of the Lp82 band (Fig. 4B, lane 4) by removal of
the N-terminal 29 amino acids as shown in Fig. 2, indicative of
activation of Lp82. This was confirmed on zymograms (Fig.
4C, lane 4) showing a smear band of active Lp82
below the usual Lp82 band. This smear band has been noted previously
during in vivo activation of Lp82 (15). These data suggested
that even when CS is present, Lp82 is not inhibited and that CS is
actually a substrate for hydrolysis by Lp82.
To determine the mechanism for the lack of inhibition of Lp82 by CS, a
three-dimensional model of Lp82 was first constructed using the crystal
structure of calpain 2 as a template (14) (Fig.
5). This was appropriate because calpain
2 and Lp82 have 51% sequence identity (7) and because the Lp82/calpain
2 match provided the best fit compared with using other templates such as papain. No significant differences between the three-dimensional structure Lp82 and calpain 2 were observed when domains IIa and b, III,
and IV from each calpain were compared against each other. Similar
results were observed when homology models of each domain were
independently compared (data not shown). However, the helical AX1
domain I of Lp82 (30.2 Å based on model) was longer than domain I of
calpain 2 (21.6 Å based on crystal structure). Since the longer
extension on domain I could influence association of Lp82 to regulatory
proteins, we also constructed a model of the association between the
traditional calpain regulatory subunit (calpain 4) and domain I in Lp82
(Fig. 6A). We found that the
longer N-terminal extension on domain I of Lp82 could interfere with
the association of Lp82 with calpain 4. This was similar to the
predicted lack of association between calpain 4 and calpain 3 (16),
possibly because of long domain I (Fig. 6B). In contrast,
because of a short domain I, calpain 2 was able to interact well with
the calpain 4 regulatory subunit (17) (Fig. 6C). For more
objective observations, VDW interaction energies were also calculated
using MOE. The VDW interaction energy between Lp82 and calpain 4 was
44,079,557 kcal/mol, and VDW contacts showing potential clashes were
observed between domain I of Lp82 and calpain 4 (Fig.
7B). Even when the Lp82 model (Lp82*) was constructed taking into account surroundings
with calpain 4, the VDW interaction energy was still high (132,181 kcal/mol), and clashes were observed between Lp82 and calpain 4 (Fig.
7C). The VDW interaction energy was also high between calpain 3 and calpain 4 (12,897,436 kcal/mol), and the clashes were
also observed (data not shown). This result was consistent with a
previous report for calpain 3 (16). In contrast, the VDW interaction
energy between calpain 2 and calpain 4 from the crystal data was only
36 kcal/mol, and no clash was observed (Fig. 7A). These data
suggested that the atoms in domain I of Lp82 and calpain 4 were too
close together to allow association between Lp82 and calpain 4.
The enormous energies (44,079,557 and 12,897,436 kcal/mol) were
homology models built and minimized without considering calpain 4 as
part of the environment. To obtain these energies, the model was left
in the MOE window, the crystal structure for calpain 4 was opened, and
there were many VDW clashes. When calpain 4 was considered part of the
environment during the model building, the calpain 4 atoms were copied
directly to the final model and included in the minimization. Thus, the
VDW interaction for Lp82* was lower (132,181 kcal/mol), since the atoms
of calpain 4 were considered present when the sequence was modeled and minimized.
A major finding of the present report was the site for autolysis
of Lp82. Our data showed that the major autolytic site was in the IS2
region. This is in contrast to the parent gene product, calpain 3, which autolyzed in the IS1 region (18). The splice deletion of IS1
apparently eliminated this autolytic site in Lp82. This is probably the
reason why Lp82 is so stable in rodent lens (12, 15) and why it retains
activity for at least 18 h in vitro (19). Unexpectedly,
we found that the N-terminal half retained activity as evidenced as the
smear band on zymograms (15). Thus, the prolonged activity of Lp82
in vitro may be due to a combination of the intact and
autolyzed active forms of Lp82. The present report also showed that
Lp82 and calpain 2 were substrates for each other. This could function
as a mechanism to down-regulate of their activities. However, in lens
Lp82 may be escape from degradation by calpain 2, because Lp82 and
calpain 2 are localized in different regions. Lp82 is concentrated in
the nucleus, while calpain 2 is concentrated in the epithelium (20).
Thus, Lp82 may provide prolonged activity in lens, even though Lp82 was
a good substrate for calpain 2 in vitro. These results
partially explain why Lp82 is the dominant calpain activity in selenite nuclear cataract (21).
The second finding of the present report was the discovery of the major
difference between Lp82 and calpain 2 interactions with endogenous
calpain inhibitor, CS. In the presence of calcium, calpain 2 was
inhibited by CS. In contrast, Lp82 hydrolyzed CS, and thus Lp82 was not
inhibited by CS. Our previous report also showed that CS domain I
(137-amino acid peptide) exhibited poor inhibitory activity against
native rat Lp82 (15). This would again favor Lp82 activity in the young
rodent lens. A similar lack of inhibition by CS occurred against
calpain 3 (16, 22). Since Lp82 and calpain 3 are from the same gene,
lack of CS inhibition could be due to similar mechanisms. CS contains
four homologous inhibitory domains. Each domain contains three regions
designated as A, B, and C (23, 24). Region B is essential for
inhibition and binds near the catalytic site in calpains 1 and 2. Regions A and C potentiate inhibitory activity by binding to domain IV of calpains 1 and 2 and to domain VI of calpain 4 (17). Our homology
model suggested that the extra amino acids in the N terminus of domain
I in calpain 3 extend into the pocket used for association of calpain 4 to calpain 2 (Fig. 6). This N-terminal extension may interfere with the
association of calpain 4 to calpain 3. Likewise, Lp82 also has unique
N-terminal sequence termed AX1, which also extends into calpain 4 binding pocket (Fig 6). This may also interfere with the association of
calpain 4 to Lp82. This was also confirmed by calculation of the VDW
interaction energies (Fig. 7).
When the calpain 4 was included in the final minimization, the VDW
interaction energy was calculated to be 132,181 kcal/mol. This shows
that many of the VDW clashes can be alleviated in the course of the
minimization; however, the interaction energy remains large. This
suggests that even with energy minimization, there is not enough room
to accommodate all of the atoms in the protein interface area without
having some atoms violate the VDW radii of others. The lack of room is
visually supported by the pictures of the interface in Fig. 6, which
shows that the extension at the N terminus of both Lp82 and calpain 3 extends from the calpain 2 template into the region where calpain 4 would normally bind.
Minimized homology models could not place the outgap residues such that
their atoms do not clash with atoms of the calpain 4. This could
explain the high VDW interaction energies observed when the outgap
residues were placed. During the homology modeling procedure, when the
outgap residues were being modeled, the scoring of the homology model
incorporates a term that reflects the VDW interaction energy between
atoms already placed and those that are currently being placed. When
the outgap residues were not included, the interaction energy in the
presence of calpain 4 was 287 kcal/mol (data not shown), which is in
the order magnitude of the interaction energy between calpain 2 and
calpain 4 from the crystal structure (36 kcal/mol). The increase in VDW
interaction energy when the model includes the outgap residues (287 kcal/mol to 132,181 kcal/mol) again suggests that the presence of the
additional atoms contributes to VDW clashes that cannot be resolved
with minimization. The presence of these potential clashes near the protein interface suggests that the unique AX1 region of Lp82 is
responsible for blocking the calpain 4 association.
Thus, the minimization part of the homology modeling cannot relieve all
of the VDW interactions, because not enough room is present to move the
outgap residues around in the region occupied by calpain 4. All
modeling can do is minimize the number of potential VDW
clashes/contacts.
These results from homology modeling are consistent with our previous
result showing that Lp82 was only poorly inhibited by CS, even in the
presence of calpain 4 (15). As described above, inhibition of calpain 2 is potentiated by binding of CS to calpain 4 (17). In fact, rcalpain 2 used in the present experiment contained calpain 4, since the
chaperone-like effect of calpain 4 was used for producing recombinant
calpain 2 (25). The lack of calpain 4 binding to Lp82 may explain why
CS was not an effective inhibitor of Lp82, although the crystal
structure of Lp82 will be needed to fully understand the inhibition
mechanism. Lack of inhibition is important physiologically because
it would allow Lp82 to be active in lens in the presence of CS.
Furthermore, degradation of CS by Lp82 may help explain how calpain 2 escapes inhibition by CS to become active in lens.
We also hypothesize that in young rodent cataracts, influx of calcium
leads to Lp82 activation, since Lp82 has a lower calcium requirement
for activation than calpain 2 (Fig.
8).2
Lp82 cleaves CS, which eliminates inhibition of calpain 2 by CS. Both
active Lp82 and calpain 2 truncate crystallins, leading to
insolubilization and precipitation of crystallins. Oxidation enhances
precipitation of truncated crystallins (Fig. 8). Activated Lp82 may be
the most active calpain in young rodent lenses. However, four deleted
nucleotides in exon 1 produce a stop codon in the Lp82 transcripts in
man.3 However, an Lp82-like
cleavage site was observed on human We gratefully thank Dr. Debra A. Brickey and
Sean Nygaard (Oregon Health and Science University, Portland, OR) for
help in expression of recombinant Lp82 and Dr. A. Raelene Lawrence
for help in protein homology modeling using MOE (Application Scientist, Chemical Computing Group Inc., Montreal, Canada).
*
This work was supported in part by National Institutes of
Health Grant EY05786 (to T. R. S.).The costs of publication of this article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
¶
To whom correspondence should be addressed: Senju Laboratory
of Ocular Sciences, Oregon Health & Science University West Campus, 505 NW 185th Ave., Beaverton, OR 97006. Tel.: 503-533-2424;
Fax: 503-533-2427; E-mail: fukiagec@ohsu.edu.
Published, JBC Papers in Press, March 19, 2002, DOI 10.074/jbc.M200697200
2
Y. Ueda, C. Fukiage, M. Shih, T. R. Shearer, and L. L. David, unpublished data.
3
H. Ma, C. Fukiage, M. Azuma, and T. R. Shearer, unpublished data.
The abbreviations used are:
NS, N-terminal
sequence;
IS, insert region;
VDW, van der Waals;
CS, calpastatin.
Characterization and Regulation of Lens-specific
Calpain Lp82*
§¶,§,,§, and
Department of Oral Molecular Biology and
Ophthalmology, Oregon Health and Science University, Portland,
Oregon 97201 and the § Senju Laboratory of Ocular Sciences,
Senju Pharmaceutical Corporation Limited, Beaverton, Oregon 97006
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
1 flow rate. Enzyme-linked immunosorbent assay was
performed by absorbing 50 µl of each column fraction in 0.1 M NaHCO3 buffer (pH 9.3) overnight onto 96-well
flat bottom plates (Corning Glass). The wells were blocked with 5%
non-fat dry milk and incubated with Lp82 (1:1000 dilution) antibody for
1 h (12). Fractions containing Lp82 were visualized using goat
anti-rabbit alkaline phosphatase-conjugated secondary antibody and
alkaline phosphatase substrate kit (Bio-Rad). The peaks were
concentrated by ultrafiltration (Microcon 10, Millipore).
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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Fig. 1.
SDS-PAGE (A) and immunoblot
(B) for rLp82 after activation with calcium.
Lanes 1-3 in B were visualized with antibody
against a peptide sequence near the missing IS2 region of Lp82.
Lanes 4-6 were visualized with antibody against the N
terminus of Lp82. Hatched and open arrows
indicate the 60- and 22-kDa autolytic products,
respectively.
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Fig. 2.
Amino acid sequences at the autolytic sites
on rLp82 at the N terminus (A, solid
arrow) and in the IS2 region (B,
hatched arrow). Locations of both sites in the
entire sequence is in shown in C.
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Fig. 3.
SDS-PAGE of inactivated calpains proteolyzed
by activated calpain 2 or Lp82 (A). Lane
1, inactivated rLp82 + rcalpain 2 without calcium; lane
2, inactivated rLp82 + rcalpain 2 with calcium; lane 3,
inactivated rcalpain 2 + rcalpain 2 with calcium; lane 4,
inactivated rcalpain 2 + rLp82 without calcium; lane 5,
inactivated rcalpain 2 + rLp82 with calcium; and lane 6,
inactivated rLp82 + rLp82 with calcium. B and
C, immunoblots for Lp82 (B) and calpain 2 (C) with the same lane designation as above.
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Fig. 4.
Proteolysis of purified erythrocyte
calpastatin by rLp82 or by rcalpain 2 as shown by SDS-PAGE
(A) and by immunoblotting for Lp82 and calpain 2 (B). Casein zymography for calpain activities
(C). Lane 1, rcalpain 2 and calpastatin with no
calcium; lane 2, rcalpain 2 and calpastatin with calcium;
lane 3, rLp82 and calpastatin with no calcium; lane
4, rLp82 and calpastatin with calcium; lane L, total
soluble protein from rat lens, with the upper white band
indicating Lp82 activity and the lower band indicating
calpain 2 activity. For immunoblotting in B, lanes
1 and 2 were visualized with antibody against calpain
2, and lanes 3 and 4 were visualized by with
antibody against Lp82.
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Fig. 5.
Ribbon rendering of human calpain 2 (left) based on the published crystal structure of
human calpain 2 (14) and a homology model of Lp82
(right). Each shows domain I
(yellow), domain IIa (green), domain IIb
(red), domain III (purple), and domain IV
(light blue).
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Fig. 6.
Docking of calpain 4 (magenta) to Lp82 (green)
(A) or to calpain 3 (light blue)
(B) and published co-crystal structure of human
calpain 2 (red) with calpain 4 (magenta) (C) (14). In
the expanded region of calpain 4 (white square), the
residues in domain I are shown in stick form without
hydrogen (yellow).
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Fig. 7.
The VDW contacts between calpain 2 (red) (A), Lp82
(green) (B), or Lp82*
(blue) (C) and calpain 4 (magenta) shown without hydrogen. The
residues in domain I on each calpain are shown in ball and stick
form (light blue). Only the atoms within 4.5 Å of the
interface between each calpain and calpain 4 are shown. The VDW
contacts showing potential clashes are shown as yellow dotted
lines. The VDW interaction energies are also shown under each
structure. Lp82* is explained in detail under "Experimental
Procedures."
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
A crystalline (26). Thus,
another p94 splice variant may assume the function of Lp82 in human
lens.
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Fig. 8.
Hypothesis relating calpain activities to
cataract formation in rodent lenses.
ACKNOWLEDGEMENTS
FOOTNOTES
ABBREVIATIONS
REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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