Originally published In Press as doi:10.1074/jbc.M109836200 on February 26, 2002
J. Biol. Chem., Vol. 277, Issue 19, 16567-16575, May 10, 2002
Analysis of Tissue Transglutaminase Function in the Migration of
Swiss 3T3 Fibroblasts
THE ACTIVE-STATE CONFORMATION OF THE ENZYME DOES NOT AFFECT CELL
MOTILITY BUT IS IMPORTANT FOR ITS SECRETION*
Zita
Balklava
,
Elisabetta
Verderio,
Russell
Collighan,
Stephane
Gross,
Julian
Adams§, and
Martin
Griffin¶
From the Department of Life Sciences, Nottingham
Trent University, Clifton Lane, Clifton, Nottingham NG11 8NS,
United Kingdom and § Smith & Nephew Group Research
Center, Science Park, Heslington,
York YO10 5DF, United Kingdom
Received for publication, October 11, 2001, and in revised form, January 10, 2002
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ABSTRACT |
Increasing evidence suggests that tissue
transglutaminase (tTGase; type II) is externalized from cells, where it
may play a key role in cell attachment and spreading and in the
stabilization of the extracellular matrix (ECM) through protein
cross-linking. However, the relationship between these different
functions and the enzyme's mechanism of secretion is not fully
understood. We have investigated the role of tTGase in cell migration
using two stably transfected fibroblast cell lines in which expression
of tTGase in its active and inactive (C277S mutant) states is inducible through the tetracycline-regulated system. Cells overexpressing both
forms of tTGase showed increased cell attachment and decreased cell
migration on fibronectin. Both forms of the enzyme could be detected on
the cell surface, but only the clone overexpressing catalytically
active tTGase deposited the enzyme into the ECM and cell
growth medium. Cells overexpressing the inactive form of tTGase did not
deposit the enzyme into the ECM or secrete it into the cell culture
medium. Similar results were obtained when cells were transfected with
tTGase mutated at Tyr274 (Y274A), the proposed site
for the cis,trans peptide bond, suggesting that
tTGase activity and/or its tertiary conformation dependent on this bond
may be essential for its externalization mechanism. These results
indicate that tTGase regulates cell motility as a novel cell-surface
adhesion protein rather than as a matrix-cross-linking enzyme. They
also provide further important insights into the mechanism of
externalization of the enzyme into the extracellular matrix.
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INTRODUCTION |
Transglutaminases (EC 2.3.2.13) are a group of
Ca2+-dependent enzymes that catalyze the
post-translational modification of proteins through the incorporation
of primary amines into the 
-carboxamide group of glutamine
residues or by the cross-linking of proteins via
-(-glutamyl)lysine bridges (1). Proteins cross-linked as a result
of transglutaminase-catalyzed reactions are generally more resistant to
mechanical, chemical, and proteolytic breakdown. Tissue
transglutaminase (tTGase1;
type II) is the most widely distributed form of transglutaminase in
mammalian tissues (1). In addition to its ability to cross-link proteins, the enzyme can also bind and hydrolyze GTP and ATP (2, 3).
Binding of GTP/GDP to the enzyme is thought to increase the tTGase
tertiary structure stability and in a viable cell keeps the enzyme
inactive as a transglutaminase (4). It has been reported that
Ca2+ and GTP induce opposite conformational changes in the
protein tertiary structure, therefore suggesting that the
mechanism by which tTGase activity is inhibited by GTP/GDP is
essentially due to a protein conformational change that obscures access
to the transglutaminase active site (5). More recent work has also suggested that a non-proline cis peptide bond close to the
active-site cysteine (Cys277) may play a role in the
conformational changes linked to the binding of Ca2+ and/or
substrate during activation of the enzyme (6).
The ability of tTGase to create covalent protein cross-links suggests
its involvement in maintaining tissue integrity; and as a consequence,
the enzyme is thought to play an important role in various
physiological as well as pathological situations such as wound healing,
fibrosis, inflammation, and tumor metastasis (7-11). Although tTGase
was originally thought to be an intracellular enzyme, accumulating
evidence indicates that the enzyme is externalized and capable of
cross-linking a wide range of extracellular matrix (ECM) proteins,
which is thought to be important in ECM deposition/stabilization and
the cell attachment and spreading of a number of different cell types
(12-15). However, the link between ECM cross-linking and the
role of the enzyme in cell attachment and spreading is still not fully
understood. Also unknown is the mechanism of secretion of the enzyme
from cells because tTGase does not possess a leader sequence, and there
is no evidence of its glycosylation (1). It is therefore unlikely that
the enzyme follows the classical endoplasmic reticulum-Golgi secretion
route. Despite this observation, evidence for the presence of tTGase in
the ECM and on the surface of different cell types is now increasing
(12-19).
It has been recently described that tTGase mediates cell
adhesion and spreading by a mechanism that is independent of its catalytic activity (20). The mechanism proposed suggests that tTGase
mediates the interaction of integrins with fibronectin, thereby acting
as an integrin-associated co-receptor (15). The results from the latter
study suggested that complexes of tTGase with integrins are formed
inside the cell during biosynthesis, leading to its accumulation on the
surface at sites of focal adhesion points (15). It has also been
demonstrated that in cells undergoing attachment and spreading, the
enzyme is co-distributed with adhesion site markers, suggesting that
these processes may coincide with the externalization of the
enzyme (21).
tTGase has a high affinity binding site for fibronectin that is
localized to the first seven N-terminal amino acids (22); and this
binding is independent of its cross-linking activity. The deletion of
this N-terminal sequence from the tTGase gene abolishes binding of the
enzyme to fibronectin and prevents its cell-surface localization,
suggesting that secretion of tTGase from the cells could be associated
with the assembly of fibronectin fibrils (23). Other proteins lacking
the classical signal sequence but efficiently secreted from the cells
have been described to cross the membrane by a novel secretion pathway
(24-27); but in most cases, the exact mechanism is still not fully understood.
Because tTGase is involved in both cell attachment and spreading and,
through its cross-linking activity, in wound healing and tissue
fibrosis (7-11, 28), it is not unreasonable to assume that it might
also be involved in cell migration, a process that is important to a
number of cellular events, including embryogenesis, tissue repair, and
tumor invasion. To explore this, we have used 3T3 fibroblasts
transfected with a number of different tTGase constructs expressing the
catalytically active or inactive forms of tTGase. We show that tTGase
can regulate migration and that this novel function is independent of
its cross-linking activity. We also demonstrate that mutation of the
active-site cysteine prevents the enzyme from being deposited into the
ECM and that mutation of Tyr274 to Ala, thought to provide
cis rather than the preferred trans peptide bond
conformation, also leads to loss of tTGase activity and of enzyme
secretion. We therefore conclude that tTGase controls cell motility by
a process that does not require its deposition into and cross-linking
of the ECM, but by acting as a novel cell-surface binding protein.
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EXPERIMENTAL PROCEDURES |
Chemicals--
All general chemicals and tissue culture reagents
were obtained from Sigma (Dorset, UK) unless otherwise stated.
PCR Mutagenesis--
The C277S mutation was introduced into
tTGase cDNA (29) as previously described (30). The resulting mutant
tTGase cDNA was inserted into the vector pUHD10.3
(14) to generate the expression plasmid
pUHD10.3-TG277.
The Y274A mutation was introduced into tTGase cDNA using the
GeneEditor in vitro site-directed mutagenesis kit (Promega,
Southampton, UK) according to the manufacturer's protocol. Starting
with the expression vector pSG5-TG containing the full-length tTGase
cDNA (donated by P. J. A. Davies, University of Texas
Health Center, Houston, TX), the TAT codon of Tyr274 was
mutated to GCT for Ala utilizing the oligonucleotide primer 5'-AAGACCCAGCACTGGCCAGCCTTGACGCGCTGGCA-3' (antisense
orientation), which is complementary to nucleotides 940-974 of tTGase
cDNA (29) and is mutated at positions 955 and 956 (underlined). The
resulting recombinant plasmid encoding mutant tTGase was named
pSG5-TG274. The presence of the base changes was confirmed
by DNA sequencing.
Transfections--
The establishment, by cell transfection, of
Swiss 3T3 cell lines expressing catalytically active tTGase under the
control of the tetracycline-regulated system (31) has been
previously described (14). Swiss 3T3 cell lines expressing inactive
C277S mutant tTGase were generated following the same protocol.
Briefly, clone tTA2, stably expressing the tetracycline-controlled
transactivator (14), was cotransfected with pUHD10.3-TG277
and the xanthine-guanine phosphoribosyltransferase expression plasmid
pUS1000 (donated by P. Sanders, University of Surrey) in the presence
of tetracycline in the medium. Clones resistant to selection medium for
the salvage enzyme xanthine-guanine phosphoribosyltransferase were
analyzed for their capacity to overexpress tTGase antigen by
standard Western blotting of cell homogenates using
anti-tTGase monoclonal antibody Cub7402 (Neomarkers).
Transfection of Swiss 3T3 fibroblasts with wild-type and inactive Y274A
mutant tTGases was achieved by cotransfecting 0.5 × 106 cells with 4.5 µg of plasmid vector
pSG5-TG274 and 0.5 µg of selection vector
pSV2neo using the liposome-based transfection reagent
ESCORTTM (Sigma) following the manufacturer's protocol.
Clones resistant to 800 µg/ml active G418 (Geneticin, Calbiochem)
were screened for overexpression of tTGase by Western blotting as
described below.
Cell Culture--
Cell lines of Swiss 3T3 fibroblasts expressing
catalytically active tTGase (clone TG3) (14) or inactive C277S mutant
tTGase (clone TGI19) in a tetracycline-regulated manner were cultured as described (14). Cell lines were continuously cultured in the
presence of tetracycline (2 µg/ml) in the medium. Under this condition, they expressed only low levels of endogenous tTGase. To
induce maximum expression of transfected tTGase cDNA, cells were cultured in the absence of tetracycline for 72 h. Cell
lines of Swiss 3T3 fibroblasts (clones TG1, TG16, TGY274A1,
TGY274A2, neo1, and neo3) expressing active or inactive
Y274A mutant tTGase or the selection marker for G418 resistance,
under the control of a non-inducible promoter, were grown in
Dulbecco's modified Eagle's medium containing 10% heat-inactivated
fetal calf serum, 2 mM glutamine, 100 units/ml penicillin,
100 µg/ml streptomycin, and 400 µg/ml G418.
Cell Migration--
The cell migration assay used was a
modification of the technique described by Akiyama et al.
(32). Low-melting-point agarose (0.2% (w/v) final concentration),
maintained just above 38 °C, was added to a suspension of cells
(3.3 × 107 cells/ml) in bicarbonate-free Dulbecco's
modified Eagle's medium (buffered with 25 mM Hepes, pH
7.4). Droplets (0.5 µl) of the cell/agarose mixture were seeded in
the center of the fibronectin (15 µg/ml)-coated wells of a 96-well
plate. After the agarose was allowed to set for 7 min at +4 °C, 100 µl of the growth medium was added to each well. In some cases, the
growth medium was supplemented with anti-tTGase antibody or tTGase
inhibitors. Cells were left to migrate for 48 h and then fixed and
stained with 0.5% (w/v) crystal violet in 70% (w/v) ethanol as
described below. The area of outwardly migrating cells was measured
using an Optimas 5.2 image analysis system (DataCell Ltd., Yately, UK).
Cell Attachment--
Cell attachment was evaluated as previously
described (13). Briefly, 100 µl of a cell suspension (5 × 105 cells/ml) was seeded in a 96-well plate coated with 5 µg/ml fibronectin, incubated in serum-free medium, and allowed to
attach for 30 min. After this, the cells were gently washed with
phosphate-buffered saline (PBS), and attached cells were fixed and
stained by addition of 0.5% (w/v) crystal violet in 70% (v/v) ethanol
at 100 µl/well. Following three washes with PBS to remove nonspecific
staining, cells were solubilized by adding 30% (v/v) acetic acid at
100 µl/well. The absorbance of the solubilized cell mixture was read at 540 nm in a SpectraFluor plate reader (Tecan).
Transglutaminase Activity Assay--
The activity of tTGase in
cell homogenates was measured by the incorporation of
14C-labeled putrescine (Amersham Biosciences,
Buckinghamshire, UK) into N,N'-dimethylcasein as
previously described by Lorand et al. (33). One unit of
tTGase activity equals 1 nmol of putrescine incorporated per h. The
activity of tTGase associated with the extracellular surface of live
cells in culture was measured by the incorporation of biotinylated
cadaverine into deoxycholate-insoluble fibronectin using an assay
described in detail by Jones et al. (13).
Detection of tTGase in Cell Fractions and Growth Medium--
For
detection of tTGase in cell homogenates, after cell lysis in ice-cold
buffer (0.25 M sucrose, 2 mM EDTA, and 5 mM Tris-HCl, pH 7.4) containing protease inhibitors (1 µg/ml pepstatin, 1 µg/ml leupeptin, and 1 mM
phenylmethylsulfonyl fluoride) and sonication, cell homogenates were
mixed with 2× Laemmli loading buffer (34) and boiled for 5 min at
100 °C, and then proteins were resolved as described below. For
separation of membrane and cytosolic fractions, cell homogenates were
first fractionated by ultracentrifugation at 100,000 × g for 1 h at +4 °C. The precipitated pellets were washed once with the cell lysis buffer and centrifuged as described above. Proteins were resolved by SDS-PAGE under reducing conditions according to Laemmli (34), and tTGase was detected by Western blotting
using anti-tTGase monoclonal antibody Cub7402 and revealed by enhanced
chemiluminescence (Amersham Biosciences) after incubation with an
anti-mouse horseradish peroxidase conjugate. For direct comparison of
cell homogenates or subcellular fractions, equal amounts of protein
were loaded onto the gels prior to fractionation.
To detect tTGase secreted into the growth medium, confluent cells were
grown in serum-free AIMV culture medium (Gibco) for 8 h. The
medium was then collected and centrifuged to remove any floating cells.
Proteins from the cell growth medium were precipitated by addition of
trichloroacetic acid to a final concentration of 10% (w/v), followed
by centrifugation. The protein pellet was washed once with 10% (w/v)
trichloroacetic acid followed by ethanol/acetone (1:1) and acetone,
dried, and resuspended in Laemmli buffer (34). The presence of tTGase
in the protein pellet was detected by Western blotting as outlined
above. Alternatively, the cell growth medium was lyophilized,
reconstituted in one-tenth of the initial volume, and analyzed for
tTGase antigen by a modified enzyme-linked immunosorbent assay (ELISA)
method according to Achyuthan et al. (35) as described below. The protein concentration was determined according to the method
of Lowry et al. (36).
Measurement of tTGase by Modified ELISA--
Detection of
extracellular tTGase was performed using the modified ELISA technique
described previously (19). Briefly, 1.5 × 104
cells/well were seeded in a 96-well plate 1 day prior to the assay.
Anti-tTGase antibody Cub7402 was diluted 1:1000 in the cell growth
medium and added directly to cells in live culture. After a 3-h
incubation, cells were washed with PBS and fixed in methanol. The
antigen-antibody complex was revealed by incubation with horseradish
peroxidase-conjugated anti-mouse IgG secondary antibody. Bound
horseradish peroxidase activity was detected by addition of
3,3',5,5'-tetramethylbenzidine substrate. Color development was stopped
with 2.5 N H2SO4, and the
absorbance was read at 450 nm in a plate reader. For protein
quantification, identical cell numbers were grown in parallel and
solubilized in 0.1% (w/v) deoxycholate. Proteins were precipitated in
10% (w/v) trichloroacetic acid and assayed by the bicinchoninic acid
method (37). The measured tTGase protein was then expressed as
A450 nm/1.0 mg of deoxycholate-soluble protein.
For detection of total tTGase, a modification of the method of
Achyuthan et al. (35) was used. Cell homogenates were added to the fibronectin-coated wells of a 96-well plate, and the binding of
tTGase to fibronectin was allowed to proceed for 1 h at 37 °C.
Wells were then blocked with blocking buffer (5% (w/v) dried skimmed
milk in PBS, pH 7.4) and incubated with Cub7402 (diluted 1:1000
in blocking buffer) for 2 h at room temperature. After three
washes with PBS, incubation with horseradish peroxidase-conjugated anti-mouse IgG secondary antibody (diluted 1:1000 in blocking buffer)
was carried out for 2 h at room temperature. Bound horseradish peroxidase activity was measured as described above. The amount of
tTGase protein was expressed as A450 nm/1.0 mg
of total protein.
Immunohistochemical Staining for Extracellular
tTGase--
Detection of extracellular tTGase was done as previously
described (14) by staining cells in culture. Immunolabeling of tTGase
was carried out using anti-tTGase primary monoclonal antibody Cub7402
and fluorescein isothiocyanate (FITC)-conjugated anti-mouse IgG
secondary antibody. Staining was visualized by confocal fluorescent microscopy using a Leica TCSNT confocal laser microscope system (Leica
Laserechnik, Heidelberg, Germany).
Flow Cytometry--
For flow cytometry, transfected Swiss 3T3
fibroblasts were detached from tissue culture dishes with 2 mM EDTA in PBS, pH 7.4. Live non-permeabilized cells in
suspension (2 × 106 cells/ml) were stained for
cell-surface tTGase with anti-tTGase antibody Cub7402 (3 µg/ml) in
serum-free medium for 3 h at +4 °C. After washing cells with
serum-free medium and incubation with FITC-conjugated anti-mouse
IgG secondary antibody, cells were washed once more, fixed in 0.5%
(v/v) formaldehyde, and analyzed with a Dako Galaxy flow cytometer.
Values represent the mean fluorescence intensity.
Statistical Analysis--
Student's t test was used
to compare data. When p was <0.05, the difference between
sets of data was considered to be statistically different.
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RESULTS |
Characterization of Swiss 3T3 Clones Transfected with Active and
Inactive C277S Mutant tTGases under the Control of the
Tetracycline-regulated System--
The amount of tTGase antigen
expressed in cell homogenates of induced transfected cells was detected
by SDS-PAGE and Western blot analysis. The Western blot shown in Fig.
1A shows clear induction of
both forms of the enzyme in TG3
and TGI19.
Densitometric analysis indicated that expression of clone TG3 increased
between 7- and 10-fold, as previously documented (14). For the inactive
C277S mutant, quantitation of induction by densitometry was not
possible because of the low endogenous background. Measurement of
antigen by a modified ELISA that first involves attachment of
the enzyme to a fibronectin-coated plate indicated a 2-3-fold induction for clone TG3 and a 4-5-fold increase for clone TG19. Overexpression of the active form of the enzyme in clone TG3 led to an
increase in total tTGase activity in cell homogenates (~12-fold) as
measured by the [14C]putrescine incorporation assay (Fig.
1C) and an increase in cell surface-related extracellular
activity (~3-4-fold) as measured by the cell-mediated incorporation
of biotinylated cadaverine into fibronectin (Fig. 1D) (14).
As expected, no tTGase activity was observed in clone TGI19 when
induced to overexpress the inactive form of the enzyme (Fig. 1,
C and D).
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Fig. 1.
Characterization of Swiss 3T3 fibroblast
clones TG3 and TGI19 displaying regulated expression of tTGase.
A, detection of tTGase antigen in cell homogenates by
SDS-PAGE analysis and Western blotting. B, measurement of
tTGase antigen in cell homogenates by the modified ELISA method.
C, measurement of tTGase activity by
[14C]putrescine incorporation into
N,N'-dimethylcasein. D, measurement of
cell surface-related tTGase activity by incorporation of biotinylated
cadaverine into fibronectin. TG3 and TGI19
are clones induced to overexpress active and inactive
tTGases, respectively, by removal of tetracycline from the
culture medium, TG3+ and TGI19+ are non-induced
controls grown in tetracycline-containing medium. Results represent
means ± S.D. from three separate experiments.
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Migratory Ability of Transfected Swiss 3T3 Fibroblasts on
Fibronectin--
By the agarose droplet method (Fig. 2A),
the transfected clone TG3 overexpressing tTGase showed a decreased rate
of cell migration on fibronectin compared
with the non-induced control (Fig. 2B), suggesting that
increased expression of tTGase affects cell motility. A reduced rate of
migration was also observed in clone TGI19 induced to overexpress
inactive tTGase compared with the non-induced cells (Fig.
2B), indicating that cell motility is not dependent on the cross-linking activity of tTGase. Interestingly, the reduction in
migration in the inactive and active clones reflected the relative amounts of induced tTGase present (see Fig. 1).
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Fig. 2.
Migration of transfected Swiss 3T3
fibroblasts. A, an example of outwardly migrating cells
from an agarose droplet. B, quantification of the
migration of fibroblasts expressing different levels of catalytically
active and inactive tTGases. C, effect of tTGase inhibitors
(10 mM putrescine, 1 mM cystamine, 0.05 mM monodansylcadaverine, 2 mM methylamine,
and 0.1 mM Rob283) on the migration of clone
TG3+. D, effect of anti-tTGase antibody on
the migration of cells from clone TG3+ treated with
increasing concentrations (mg/ml) of Cub7402 (shaded bars)
or control nonspecific mouse IgG (hatched bars).
TG3 and TGI19 are clones induced to
overexpress active and inactive tTGases, respectively; TG3+
and TGI19+ are non-induced controls. Results represent
means ± S.D. from three independent experiments. *, significant
difference (p < 0.05) between induced clones and
non-induced controls.
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When left to migrate in the presence of a range of competitive
substrates of tTGase, the motility of TG3 cells was not significantly affected compared with that of untreated cells (Fig. 2C).
Similarly, cell motility was also not affected when the irreversible
active site-specific inhibitor Rob283
(2-[(2-oxopropyl)thio]imidazolium derivative) (38, 39) was used
at a concentration of 0.1 mM (IC50 ~ 50 µM in our hands) (Fig. 2C), further suggesting
that the cross-linking activity of the enzyme is not responsible for the observed effect of tTGase on cell migration.
To explore whether the intracellular or extracellular fraction of
tTGase was affecting cell motility, cell migration was assessed in the
presence of varying amounts of mouse anti-tTGase monoclonal antibody
Cub7402, which binds to cell-surface tTGase as previously shown (13,
14). Addition of Cub7402 to non-induced TG3 cells decreased the rate of
fibroblast migration in a dose-dependent manner (Fig.
2D), and migration was completely abolished at 0.1 mg/ml. Cells treated with control mouse IgG showed a migration rate
similar to that of the untreated cells. This indicates that the major
candidate involved in migration is cell surface-related tTGase.
Attachment of Transfected Swiss 3T3 Fibroblasts--
Cells induced
to overexpress tTGase (active and inactive C277S mutant) demonstrated a
small but significantly greater attachment to fibronectin-coated
surfaces than the non-induced controls when cultured in serum-free
medium (Fig. 3). This effect was not
observed when cells were seeded on tissue culture plastic in the
presence of serum-containing medium (data not shown).
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Fig. 3.
Effects of tTGase on cell attachment.
The number of cells attached in 30 min to fibronectin-coated surfaces
was measured by staining cells with crystal violet as described under
"Experimental Procedures." TG3 and
TGI19 are clones induced to overexpress active and
inactive tTGases, respectively; TG3+ and TGI19+
are non-induced controls. Results represent means ± S.D. from
three separate experiments. *, significant difference
(p < 0.05) between induced clones and non-induced
controls.
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Cellular Localization of tTGase in Transfected Cells--
In view
of the findings shown in Figs. 2 and 3, it was important to demonstrate
that inactive C277S mutant tTGase has a subcellular distribution
comparable to that of the active wild-type enzyme. To explore the
subcellular distribution of tTGase in the different transfected cells,
cell homogenates were initially fractionated by centrifugation, and the
cytosolic and membrane-rich fractions were analyzed by Western
blotting. The active form of the enzyme could be found in both the
cytosolic and membrane fractions of cells expressing endogenous levels
of enzyme (TG3+) (Fig. 4).
However, following induction, both forms of the enzyme (TG3 and TGI19) could be detected in the
membrane and cytosolic fractions (Fig. 4).
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Fig. 4.
Western blot analysis of the cellular
distribution of tTGase in transfected clones. TG3
and TGI19 are clones induced to overexpress active and
inactive tTGases, respectively; TG3+ and TGI19+
are non-induced controls. Cells were fractionated into membrane-rich
(M) and cytosolic (C) fractions as described
under "Experimental Procedures."
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Immunochemical staining of cells for matrix-associated
tTGase (14) indicated increased ECM-associated enzyme in
induced cells overexpressing the catalytically active form of the
enzyme. In contrast, cells displaying increased expression of inactive C277S mutant tTGase showed levels of externalized enzyme comparable to
those of the non-induced cells or cells incubated with nonimmune mouse
IgG (Fig. 5A), suggesting that
this inactive form of the enzyme is not secreted and deposited into the
ECM. Use of an ELISA-based method to quantify extracellular tTGase (19)
confirmed that an increased level of ECM-associated tTGase could be
detected only in cells overexpressing the active form of the enzyme and not in cells overexpressing the inactive form of tTGase compared with
non-induced cells (Fig. 5B).
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Fig. 5.
Detection of the extracellular pool of tTGase
in transfected 3T3 fibroblasts. A, immunofluorescent
staining of extracellular tTGase in cultured transfected fibroblasts.
The Cub7402 antibody or nonimmune mouse IgG was added to live cell
cultures, and the immunofluorescence of FITC-conjugated secondary
antibody was detected by confocal microscopy as described under
"Experimental Procedures." Bar = 50 µm.
B, measurement of ECM-associated tTGase by a modified ELISA
as described under "Experimental Procedures." TG3 and
TGI19 are clones induced to overexpress active and
inactive tTGases, respectively; TG3+ and TGI19+
are non-induced controls. Absorbance levels were normalized to 1 mg of
deoxycholate-extracted protein. Results represent means ± S.D.
from three separate experiments. *, significant difference
(p < 0.05) between induced clones and non-induced
controls.
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Western blot analysis of both induced clones TG3 and
TGI19 showed an increased presence of active and inactive
tTGases, respectively, in the cell membrane fraction. The presence of
both forms of tTGase on the cell surface was confirmed by immunoprobing
the cell surface, followed by flow cytometry analysis. These results
showed that induced cells overexpressing both active and inactive C277S
mutant tTGases had increased levels of surface enzyme compared with
their non-induced controls (Fig. 6). The
relative amount of enzyme on the cell surface appeared to be comparable
to the total level of enzyme present in the clones (see Fig. 1).
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Fig. 6.
Analysis of the cell-surface enzyme found in
transfected clones by flow cytometry. Cells were detached with
EDTA and incubated in suspension with primary antibody Cub7402,
followed by incubation with FITC-conjugated secondary antibody as
described under "Experimental Procedures." TG3 and
TGI19 are clones induced to overexpress active and
inactive tTGases, respectively; TG3+ and TGI19+
are non-induced controls. Mouse IgG was used as the isotype control and
for setting of the background gate.
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Detection of tTGase in the Cell Growth Medium--
Because the
inactive C277S mutant enzyme may be deposited into the cell culture
medium rather than the ECM, the cell growth medium was also analyzed.
To avoid the binding of externalized tTGase to serum fibronectin, cells
were incubated in serum-free AIMV medium for 8 h prior to analysis
of tTGase antigen. Analysis of proteins precipitated from the growth
medium by Western blotting indicated the presence of tTGase antigen in
the medium of clone TG3, induced to express the active
form of the enzyme (Fig. 7A). In contrast, tTGase could not be detected in the medium of the non-induced cells (TG3+ and TGI19+) or cells
overexpressing the inactive C277S mutant form of the enzyme
(TGI19) (Fig. 7A). This result was confirmed
when the cell growth medium was analyzed by the modified ELISA (Fig.
7B).
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Fig. 7.
Measurement of tTGase in serum-free AIMV cell
culture medium after an 8-h incubation. A, Western blot
showing the presence of tTGase in the cell culture medium after
precipitation of proteins with trichloroacetic acid as described under
"Experimental Procedures." B, measurement of tTGase
antigen in 10× concentrated AIMV serum-free cell culture medium
by a modified ELISA as described under "Experimental Procedures."
TG3 and TGI19 are clones induced to
overexpress active and inactive tTGase respectively; TG3+
and TGI19+ are non-induced controls. AIM V, 10×
concentrated serum-free AIMV cell culture medium; TGstd,
guinea pig liver transglutaminase standard. Results represent
means ± S.D. from three separate experiments. *, significant
difference (p < 0.05).
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Characterization of Swiss 3T3 Clones Transfected with Active and
Inactive Y274A Mutant tTGases--
Our data so far indicate that
transglutaminase activity and/or an active-site region containing a
Cys277 rather than a Ser277 mutation is
required for externalization of the enzyme into the surrounding matrix.
Recent studies (6) have shown that also present in this active-site
region of tTGase at Tyr274 is a peptide bond held in the
cis conformation, and not in the favored trans
conformation. Given the closeness of this cis peptide bond
to the active-site Cys277, there is the possibility that
mutation of Cys277 to Ser could affect this cis
conformation as well as nullify transglutaminase activity. The question
therefore arises whether the mutation of Tyr274, which
stabilizes the cis peptide bond conformation (6), to Ala274 also affects externalization of the enzyme. To
address this question, codon 274 of the tTGase cDNA was mutated to
encode Ala by site-directed mutagenesis, and the Y274A mutant and
wild-type cDNAs were then stably expressed in Swiss 3T3
fibroblasts. Analysis of the expressed enzyme in transfected clones by
Western blotting (Fig. 8A) and by the modified ELISA (Fig. 8B) indicated that the
tTGase-transfected clones (wild-type TG1 and TG16 and Y274A mutant
TGY274A1 and TGY274A2) showed increased amounts
of tTGase expression compared with the transfected negative controls
(neo1 and neo3 expressing the selection vector pSV2neo
only). The Y274A mutation did not affect binding to fibronectin, as the
active and inactive mutant tTGases showed comparable
fibronectin-binding abilities (Fig. 8B) in the modified ELISA. Overexpression of the active form of the enzyme in clones TG1
and TG16 led to an increase in tTGase activity in total cell homogenates (Fig. 8C) and an increase in cell
surface-related extracellular activity (Fig. 8D). However,
as expected (6), the mutation at position 274 diminished tTGase
activity in clones TGY274A1 and TGY274A2,
comparable to that in the transfected negative controls (neo1 and neo3)
(Fig. 8, C and D).
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[in a new window]
|
Fig. 8.
Characterization of Swiss 3T3 clones
transfected with active and inactive Y274A mutant tTGases.
A, detection of tTGase antigen in cell homogenates by
SDS-PAGE analysis and Western blotting. B, measurement of
tTGase antigen in cell homogenates by the modified ELISA
method. C, measurement of tTGase activity by
[14C]putrescine incorporation into
N,N'-dimethylcasein. D, measurement of
cell surface-related tTGase activity by incorporation of biotinylated
cadaverine into fibronectin. TG1 and TG16 are clones transfected with
active wild-type tTGase; TGY274A1 and TGY274A2
are clones transfected with inactive Y274A mutant tTGase; and neo1 and
neo3 are transfected negative controls. Results for A,
C, and D represent means ± S.D. from three
separate experiments.
|
|
Cellular Localization and Externalization of Y274A Mutant
tTGase--
To investigate the effect of the Y274A mutation on enzyme
externalization, the transfected clones were first fractionated by
centrifugation, and cytosolic and membrane-rich fractions were analyzed
by Western blotting. The active and inactive Y274A mutant forms of the
enzyme could be found in both the cytosolic and particulate fractions
of cells, but the mutant form of tTGase showed a smaller amount of
enzyme associated with the cell membrane fraction compared with active
tTGase (Fig. 9).
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Fig. 9.
Western blot analysis of the cellular
distribution of tTGase in transfected clones. Cells were
fractionated into membrane-rich (M) and cytosolic
(C) fractions as described under "Experimental
Procedures." TG1 and TG16 are clones transfected with active
wild-type tTGase; TGY274A1 and TGY274A2 are
clones transfected with inactive Y274A mutant tTGase; and neo1 and neo3
are transfected negative controls.
|
|
Transfected clones were also immunoprobed for the presence of tTGase on
the cell surface and analyzed by flow cytometry. In keeping with the
fractionation studies (Fig. 9), clones expressing the active form of
tTGase (TG1 and TG16) showed increased amounts of cell-surface enzyme
compared with the transfected negative controls (neo1 and neo3) (Fig.
10). Clones transfected with Y274A mutant tTGase (TGY274A1 and TGY274A2) showed
only a small increase in the amount of cell-surface enzyme compared
with the transfected negative controls (neo1 and neo3) (Fig. 10).
Unlike active tTGase, the Y274A mutant form of tTGase could not be
detected in the cell growth medium (Fig.
11) when analyzed by Western blotting,
indicating that it is unlikely to be secreted from cells.
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Fig. 10.
Analysis of the cell surface-related enzyme
in cells transfected with the Y274A mutant and the respective controls
by flow cytometry. Cells were detached with EDTA and incubated in
suspension with primary antibody Cub7402, followed by incubation with
FITC-conjugated secondary antibody as described under "Experimental
Procedures." TG1 and TG16 are clones transfected with active
wild-type tTGase; TGY274A1 and TGY274A2 are
clones transfected with inactive Y274A mutant tTGase; and neo1 and neo3
are transfected negative controls. Labeling with mouse IgG was used as
the isotype control and for setting the background gate.
|
|
View larger version (49K):
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|
Fig. 11.
Detection of active wild-type and inactive
Y274A mutant tTGases in serum-free AIMV cell culture medium after an
8-h incubation. A Western blot shows the presence of tTGase in
serum-free AIMV cell culture medium after precipitation of proteins
from the medium with trichloroacetic acid as described under
"Experimental Procedures." TG1 and TG16 are clones transfected with
active wild-type tTGase; TGY274A1 and TGY274A2
are clones transfected with inactive Y274A mutant tTGase.
|
|
| |
DISCUSSION |
The functional role played by tTGase in cell migration has never
been clearly established despite observations indicating that tTGase is
involved in cell adhesion (14, 15, 29, 41). In this report, our
objective was to ascertain whether the enzyme's effect on cell
migration was due to its cross-linking activity, its action as a
cell-surface binding protein, and/or its ability to act as a
GTP-binding protein. The model used involved cell lines of Swiss 3T3
fibroblasts expressing catalytically active or inactive C277S mutant
tTGase in a tetracycline-regulated manner. We have previously shown
that this model allows maximum expression of tTGase following a 72-h
period of induction (14, 19, 23). It does not suffer from clonal
variation because each clone acts as its own control when induced;
moreover, it gives homogeneous enzyme expression unlike the
heterogeneous expression and low transfection efficiency often
associated with transient transfection models.
In transfected cells induced to express catalytically active tTGase
(clone TG3), the activity of tTGase was increased in cell homogenates
and at the cell surface of the cells, confirming that increased
expression of tTGase leads to increased externalization of the enzyme
as previously found (14). Following induction of catalytically inactive
C277S mutant tTGase in clone TGI19, the tTGase activity of cell
homogenates remained unchanged, as expected. The relative measure of
the ability of the C277S mutant and wild-type proteins in the
transfected cell lines to associate with the substrate fibronectin was
found to be comparable. This is a significant result in support of our
additional investigations, as we have recently shown that binding of
tTGase to fibronectin is crucial for enzyme cell-surface localization
(23). We demonstrated that fibroblasts induced to overexpress active
and inactive forms of tTGase showed a decreased rate of migration on
fibronectin, which was accompanied by enhanced cell attachment,
suggesting that the cross-linking activity of tTGase is not responsible
for the enzyme's effects on cell motility. This observation was
confirmed by the inability of inhibitors of tTGase activity to affect
cell migration. One of these inhibitors, the irreversible inhibitor Rob283, led to ~90% inhibition of cell surface-related tTGase activity when used at 100 µM (data not shown). However,
the ability of anti-tTGase monoclonal antibody Cub7402 to reduce cell
migration in a dose-dependent manner indicates that the
cell-surface enzyme is an essential component in the migration of
cells. Complete loss of cell motility at 100 µg/ml Cub7402 could be
explained by earlier findings indicating that the binding of the
antibody to cell-surface tTGase completely inhibits cell attachment to fibronectin (14). As a consequence, cell movement is not possible without cell attachment. This ability of anti-tTGase antibodies to
block both cell attachment and cell migration is comparable to the
outcome observed when cells are incubated with antibodies directed
against the cell-surface region of the 
1- and
5-integrins (42). Integrin ligand-binding properties are
thought to govern cell migration speed through the degree of
cell-substratum adhesiveness (43). The data reported here indicate that
the effects of tTGase on the migration of fibroblasts are brought about
by a similar mechanism. Our studies on cell attachment to fibronectin
show that overexpression of tTGase (active and inactive forms), which was accompanied by a decreased rate of cell migration, led to a small
but significant increase in cell adhesiveness. Previous work has also
demonstrated that changes in expression of tTGase in NIH 3T3
fibroblasts (44), fibrosarcoma cells (45), and endothelial like cells
(13) can lead to similar changes in cell adhesion.
Using immunogold electron microscopy, we have recently provided
evidence for a preferential extracellular location of tTGase in dense
clusters close to the cell surface/pericellular matrix and in
association with fibronectin (23). It is therefore possible that tTGase
might be involved in cell attachment and migration as a cell-surface
binding protein. In agreement with our data, Akimov et al.
(15) recently reported that the adhesive function of tTGase does not
require its cross-linking activity, but is thought to be dependent on
its stable noncovalent association with integrins. A close association
of tTGase with 1-integrin was also demonstrated by
Gaudry et al. (21) in the early stages of cell attachment by
immunofluorescent staining. However, in this case, the localization
became less prominent as cells spread more. Therefore, tTGase could
function as a cell-surface molecule independent of its catalytic
activity, directly through its close association with fibronectin (23),
or by interacting with the integrin cell-surface receptors (15),
promoting cell interaction with the matrix and therefore slowing down
cell migration. Alternatively, tTGase could still act as a GTP-binding
protein in controlling cell migration (the C277S mutant retains
GTP-binding activity), although the ability of cell surface-directed
anti-tTGase antibodies to block migration strongly suggests it to be a
cell-surface event.
In previous work using 96-h-old cultures of Swiss 3T3 cells induced to
overexpress tTGase, we reported a clear increase in -(-glutamyl)lysine cross-links, the majority of which are likely to be present in the ECM (14). It may therefore be plausible that
tTGase contributes early to cell adhesion, acting from the cell surface
independent of its cross-linking activity; but once released in the
extracellular space, possibly by a "piggyback" mechanism via its
binding to fibronectin, it starts to accumulate and in doing so
contributes to the cross-linking of ECM proteins when and if
appropriate substrates become available. This suggests that
stabilization of ECM proteins by tTGase is more of a "long-term" process as a result of the progressive accumulation of secreted tTGase
and availability of substrate proteins rather than an immediate event
capable of mediating cell adhesion and migration. However, in a
pathological situation such as in a wounded area, an increased amount
of tTGase might also be deposited into the matrix as a result of
increased expression of the enzyme (10) or as a result of leakage
following cell stress (28) or cell death and exert its
cross-linking-mediated role of matrix stabilizer directly, thus
contributing to the maintenance of tissue integrity.
Important to the hypothesis that a cell surface-related
tTGase (active or inactive) can mediate changes in cell
migration is that both the active and inactive C277S mutant enzymes
have similar cellular distributions and that mutation of the enzyme does not affect this distribution. Our data show that both forms of
tTGase were detected at the cell surface. However, only cells overexpressing the catalytically active form of tTGase showed increased
and detectable amounts of tTGase antigen deposited into the ECM and
culture medium. This novel finding indicates that only cell
surface-associated tTGase and not tTGase deposited into the matrix is
required to affect the cell migratory process; moreover, this function
of tTGase does not require cross-linking activity. Our preliminary
studies have indicated so far that incubation of cells with the active
site-directed inhibitor Rob283 or the competitive primary amine
cystamine did not significantly reduce the amount of enzyme deposited
into the matrix (data not shown). This initially suggests that the
cross-linking activity of the enzyme is not required for the complete
secretory process. However, these inhibitors may not access the active
site until the enzyme is in its Ca2+-mediated active
conformation, which is when the enzyme is already at the cell surface.
We therefore cannot rule out that the active-site Cys277
has two important roles in the secretory mechanism: one that is
essential to the folding of the protein to achieve a conformation necessary for the secretion and the other in the cross-linking mechanism of the enzyme.
Recently, on the basis of crystallographic studies of
Factor XIIIa, a novel mechanism for transglutaminase activation has been proposed based on the identification of two non-proline
cis peptide bonds, which are thought to act as a
conformational switch between catalytically active/inactive states of
transglutaminase (6). In Factor XIIIa, one of these bonds is thought to
be necessary for close association of the two active
a subunits, whereas the other is close to the
active-site cysteine. According to this work, the conformational
rearrangements necessary to expose the hidden active site would depend
on the cis-to-trans isomerization of these
peptide bonds, which may be linked to substrate, or calcium binding.
The fact that these bonds are very rare in protein structures (46) and
that one of them is found close to the active site, which is a highly
conserved region among transglutaminases, strongly suggests a
functional role for them. We therefore transfected Swiss 3T3 cells with
tTGase in which the potential tTGase cis peptide close to
the active-site region at position 274 was mutated from Tyr to Ala
(Y274A). Analysis of these transfected cells indicated that the Y274A
mutation abolished the activity of tTGase in both clones examined, as
previously predicted (6). Comparison of wild-type clone TG16 and mutant
clone TGY274A2, which express similar amounts of total
enzyme, indicated that both the active and inactive Y274A mutant forms
of the enzyme could be found in the membrane-rich and cytosolic
fractions of the cells; however, cells expressing the mutant form of
tTGase showed lower levels of membrane-associated enzyme. Measurement
of cell-surface tTGase by flow cytometry confirmed that the clones
expressing the Y274A mutant form of the enzyme had relatively small
amounts of cell-surface tTGase, although the levels were greater than
those in the transfected negative controls (neo1 and neo3). The Y274A
mutation was also found to prevent secretion of the enzyme into the
cell culture medium.
Our data therefore show that mutations in the Cys277
active-site region of the enzyme and at Tyr274, which lies
in a newly predicted non-proline cis peptide bond region
thought to be critical for the exposure of the enzyme active site, both
lead to loss of cross-linking activity. We also demonstrate that the
conformation of this active-site region of the enzyme or possibly the
cross-linking activity of the enzyme is a major factor in the mechanism
that governs the secretion and deposition of the enzyme into the ECM.
Hence, secretion of the enzyme may be connected to the
cis-to-trans isomerization of the non-proline cis peptide bonds. We hypothesize that the active
trans conformation may occur in the enzyme upon the binding
of Ca2+ and substrate. This process would occur once the
enzyme reaches the cell surface, where both Ca2+ and
substrates such as fibronectin are available to the enzyme. Interestingly, we have recently reported that the fibronectin-binding site in the N-terminal -sandwich domain of tTGase is also important in the secretion mechanism of this enzyme (23).
In conclusion, this work shows the importance of
cell-surface tTGase in the regulation of cell migration. This novel
function of the enzyme does not require tTGase catalytic activity and
can be correlated with a tTGase-mediated increase in cell adhesion strength. We have also demonstrated for the first time that the active-site cysteine and the tertiary structure of the active-site region, including a putative non-proline cis peptide bond,
are key players in determining enzyme secretion.
| |
ACKNOWLEDGEMENTS |
We thank John Bladon (Rotherham General
Hospital) for help with flow cytometry and Rob Saint and Ian Coutts
(Nottingham Trent University) for synthesis of the transglutaminase
inhibitor Rob283.
| |
FOOTNOTES |
*
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. Tel.:
44-115-8486670; Fax: 44-115-8486636; E-mail:
martin.griffin@ntu.ac.uk.
Published, JBC Papers in Press, February 26, 2002, DOI 10.1074/jbc.M109836200
| |
ABBREVIATIONS |
The abbreviations used are:
tTGase, tissue
transglutaminase;
ECM, extracellular matrix;
PBS, phosphate-buffered
saline;
ELISA, enzyme-linked immunosorbent assay;
FITC, fluorescein isothiocyanate.
| |
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111,
699-708[Abstract/Free Full Text] |
TOP
ABSTRACT
INTRODUCTION
