Department of Dermatology, Washington University Medical School, St. Louis, Missouri 63110
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Abstract |
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We examined intercadherin interactions in
epithelial A-431 cells producing endogenous E-cadherin and recombinant forms of E-cadherin tagged either by myc or by flag epitopes. Three distinct E-cadherin complexes were found. The first is a conventional
E-cadherin-catenin complex consisting of one E-cadherin molecule linked either to -catenin/
-catenin or
to plakoglobin/
-catenin dimers. The second is a lateral
E-cadherin complex incorporating two E-cadherin- catenin conventional complexes combined in parallel
fashion via dimerization of the NH2-terminal extracellular domain of E-cadherin. The third complex is likely
to contain two E-cadherin-catenin conventional complexes derived from two opposing cells and arranged in
an antiparallel fashion. Formation of the antiparallel
but not lateral complex strictly depends on extracellular calcium and E-cadherin binding to catenins. Double
amino acid substitution Trp156Ala/Val157Gly within
the extracellular NH2-terminal E-cadherin domain
completely abolished both lateral and antiparallel inter-E-cadherin association. These data support an idea
that the antiparallel complex has the adhesion function.
Furthermore, they allow us to suggest that antiparallel
complexes derive from lateral dimers and this complex
process requires catenins and calcium ions.
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Introduction |
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THE classic cadherins (e.g., E-, N-, and P-cadherins)
are single transmembrane domain proteins involved
in calcium-dependent homophilic cell-cell recognition and adhesion. In the intercellular adherens junctions,
cytoplasmic portions of these proteins orchestrate assembly of the electron-dense plaque that anchors microfilaments to the plasma membrane. It is thought that the resulting junctional system plays a pivotal role in the
establishment and maintenance of the unique tissue architecture (Vasiliev and Gelfand, 1981; Edelman et al., 1990
;
Takeichi, 1991
; Hynes, 1993; Gumbiner, 1996
; Hubar et al.,
1996
). Furthermore, it is now clear that classic cadherins
are important elements of the complex signaling pathways controlling cellular motility, growth, and differentiation
(Geiger and Ayalon, 1992
; Klymkowsky and Parr, 1995
;
Peifer, 1995
). Defects in cadherin-dependent intercellular
adhesion accompany neoplastic transformation and tumor
progression (Takeichi, 1993
; Birchmeier and Behrens,
1994
). Despite these critical functions, little is known
about the physical interactions between cadherin molecules leading to the establishment of cell-cell contacts, intracellular signals, or the regulation of these interactions
by extracellular or intracellular factors.
The extracellular region of classic cadherins consists of
five repeating domains (EI-EV). Together they coordinate several calcium ions that maintain the rod-like conformation of the entire extracellular region and are also
required for cadherin's adhesion activity (Ozawa et al.,
1990a; Pokutta et al., 1994
; Maurer et al., 1996
). Experiments with cadherin mutants and chimeric molecules showed that the NH2-terminal EI domain governs the
binding specificity of cadherins (Blaschuk et al., 1990
;
Nose et al., 1990
). Recently, X-ray crystallographic studies
determined the three-dimensional structure of the EI domain of N- and E-cadherin (Overduin et al., 1995
; Shapiro
et al., 1995
) and the EI-EII domains of E-cadherin (Nagar
et al., 1996
). All reports confirmed that calcium ions stabilize the interdomain organization of the extracellular cadherin region. Furthermore, analysis of cadherin crystals
suggested that these proteins may form lateral homodimers. The models of organization of such dimers, however, differed significantly in two reports. According to
one model (Shapiro et al., 1995
) two cadherin molecules extending from the same cell surface laterally interact
through hydrophobic interactions. A major feature of this
interaction is the mutual incorporation of the conserved
Trp residue, localized at the second position in mature
classic cadherins, into the hydrophobic core of the paired
molecule. This model was supported by experiments with
the recombinant extracellular portion of Xenopus C-cadherin showing that homodimerization is calcium independent (Brieher et al., 1996
). In the alternative model (Nagar
et al., 1996
), lateral cadherin dimers are stabilized by mutually coordinating calcium ions. The second model is consistent with the observation that at high concentrations the
recombinantly expressed extracellular region of mouse
E-cadherin dimerized in a calcium-dependent manner (Koch et al., 1997
). The existence of any of such dimers on
the cell surface was not confirmed by direct experiments.
Dimerization of the extracellular E-cadherin segment,
however, was demonstrated in pentameric structures assembled by chimeric proteins consisting of the extracellular portion of E-cadherin and the transmembrane region
of cartilage oligomeric matrix protein (Tomschy et al., 1996
).
It has been proposed that lateral cadherin dimers associate into antiparallel complexes that result in cell-cell adhesion (Shapiro et al., 1995). The structural basis of this interaction is not clear. Available data suggest that lateral
cadherin dimers are more efficient in adhesive interactions
than monomers and their formation may regulate intercellular adhesion (Brieher et al., 1996
; Tomschy et al., 1996
).
Extracellular calcium ions were shown to be required for
cadherin-dependent cell-cell adhesion (Kartenbeck et
al., 1982
; Volberg et al., 1986
; Ozawa et al., 1990a
). Some
evidence, however, suggested that disruption of cadherin adhesion by calcium removal may have a complex
mechanism and may be triggered via remodeling of the
microfilament cytoskeleton (Citi, 1992
; Citi et al., 1994
;
Shapiro et al., 1995
).
Another well-established feature of classic cadherins is
their interaction with cytoplasmic proteins, catenins. The
intracellular cadherin region directly interacts either with
-catenin or with plakoglobin (
-catenin). Both these proteins associate with
-catenin, which is thought to link the
cadherin-catenin complex to the actin cytoskeleton. Deletion of the catenin-binding domain completely abolished
the adhesion activity of classic cadherins (Nagafuchi and
Takeichi, 1988
; Ozawa et al., 1989
, 1990b
), and the attachment of cells to immobilized lateral cadherin dimers (Brieher et al., 1996
). A possible explanation for these observations is that association with the cytoskeleton via catenins
is an important prerequisite to the formation of E-cadherin clusters which, in turn, are required for lateral
dimerization (Tomschy et al., 1996
).
To further our understanding of classic cadherin-based
adhesion, we developed an approach allowing us to directly observe the lateral and antiparallel (adhesive) cadherin complexes. We demonstrated that a relatively small
pool of E-cadherin does form lateral homodimers. Features of these dimers are consistent with the model proposed by Shapiro et al. (1995). In addition to lateral dimers, we were able to detect adhesive complexes formed
by cadherins extending from two opposing cells. E-cadherin association with catenins was required for the formation of the adhesive but not lateral dimers. We present evidence that lateral and adhesive cadherin complexes are
the distinct and consecutive steps of cadherin-mediated adhesion and discuss a possible role of catenins in the establishment of the adhesion interactions.
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Materials and Methods |
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Cloning of Human E-cadherin and Its Mutants
Fragments of the human E-cadherin gene between nucleotides 89 and 982 (fragment 1); 756 and 1,652 (fragment 2); 1,372 and 2,363 (fragment 3);
2,105 and 2,802 (fragment 4; nucleotide and amino acid sequences of
E-cadherin are numbered accordingly to the sequence with GenBank/
EMBL/DDBJ accession number Z13009, Bussemakers et al., 1993) were
amplified by PCR from a human salivary gland cDNA (Clontech, Palo
Alto, CA) using the following pairs of primers: 5'-CCAGCCATGGGC-CCTTGGAGCCGC-3' and 5'-GTAGGTGTTCACATCATCGTCCGC-3'; 5'-ATAGAGAACGCATTGCCACATACA-3' and 5'-TCTGTTCCATAAATGTGTCTGGCT-3'; 5'-CACAAATCCAGTGAACAACGATGG-3' and 5'-CATCATAGTAATAAACGTTGTCCC-3'; 5'-GATAACCAGAATAAAGACCAAGTG-3' and 5'-GAACGCTGATTTC-TGCATTTCCCA-3'. The fragment 4 was blunt ended, cleaved by EcoRI,
and then ligated with the EcoRI-SmaI-digested Bluescript II KS+ vector
(Stratagene, La Jolla, CA). The resulting plasmid was cleaved by KpnI-EcoRI and ligated with the KpnI-EcoRI-digested fragment 3 that generates a plasmid BlEc3-4. In parallel experiments, the fragment 1 was blunt
ended, treated with BamHI, and then ligated with the BamHI-EcoRV- digested Bluescript vector. The resulting plasmid was combined with the
fragment 2 using overlapping EcoRI site that generates a plasmid BlEc1-2.
Finally, to construct the BlEcwt plasmid encoding a full-length E-cadherin
cDNA, the KpnI fragment of the plasmid BlEc1-2 was inserted into the
KpnI-cleaved BlEc3-4 plasmid. E-cadherin cDNA of this plasmid was
completely identical to the 89-2,802 nucleotide sequence of E-cadherin
published by Bussemakers et al. (1993)
.
To facilitate detection and immunoprecipitation, E-cadherin or its mutants were tagged COOH terminally by 6× myc or by a single flag
epitope. For this procedure, the BamHI site was substituted for the E-cadherin stop codon in the BlEcwt using PCR-mediated mutagenesis. This
site was used for ligation of the E-cadherin gene with the unique BamHI
site of 6× myc sequence in the plasmid CS26MT (Chitaev and Troyanovsky, 1997) or with the BglII site of the Flag sequence of the plasmid
pFLAG-CTS (Sigma Chemical Co., St. Louis, MO). PCR-mediated mutagenesis was used to construct the plasmid BlEc1M encoding E-cadherin
containing the internal deletion in the cytosolic domain between His773
and Leu791 (Ec1M). This deletion as was shown in preliminary experiments specifically eliminates the recognition site of anti-E-cadherin mAb
(clone C20820, Transduction Laboratories, Lexington, KY). To introduce
this deletion, two E-cadherin fragments (1,699-2,406 and 2,468-2,740
nucleotides) were amplified by PCR using primers 5'-TAATCCGGACACTGGT and 5'-AAACAATTGGCTCAGTCAAAGTC and 5'-AAACAATTGATGAGTGTCCCCCGGTAT and 5'-GGATCCGTCGTCCTCGCCGCCTCC. They were then ligated through the unique MunI site
(underlined) and the resulting fragment was inserted between the BspEI
and BamHI sites of the BlEc1M plasmid.
To construct the deletion mutant Ec1(159-536)M, the unique NcoI/
BspEI fragment (94-1,702 nucleotides) in the BlEc1M was replaced with
the fragment (94-573) resulting from PCR performed with primers 5'-CGGCCAGCCATGGGCCCT and 5'-AAAGTCCGGAGGAATAACCCAGTCTCT. Plasmids BlEc1
(772-882) and BlEc1
(748-882) encoding two different COOH terminally truncated E-cadherin mutants were
also constructed using PCR. The BspEI/BamHI fragment (1,703-2,745) of
the BlEc1M plasmid was replaced with the fragments amplified between
1,699 and 2,410 or between 1,699 and 2,339 nucleotides of E-cadherin cDNA, respectively. Identical sense primer 5'-TAATCCGGACACTGGT and different antisense primers 5'-AAAGGATCCCAGCTGGCTCAAGTC and 5'-AAAGGATCCGGTGTATCCTCTGGGGG were used.
PCR-mediated mutagenesis was also used to introduce point mutations. In
the mutant Ec1WVM, a nucleotide sequence GACTGGGTT encoding the
Asp155TrpVal amino acid sequence was replaced with GACGCCGGC, resulting in a new NaeI site. In the mutant Ec1QNM, the nucleotide sequence GATCAGAAT encoding Asp254GlnAsn tripeptide was replaced
with GATGCTGCA. For transfection of A-431 cells, the corresponding
Bluescript clones were further subcloned into the eukaryotic expression
vector pRcCMV (Invitrogen, Carlsbad, CA) containing a neomycin resistance gene and cytomegalovirus (CMV) promoter.
The integrity of the constructs was confirmed by restriction endonuclease mapping. All fragments obtained by PCR were completely sequenced using the sequencing core facility of Washington University Medical School (St. Louis, MO).
Cell Culture, DNA Transfection, and Immunofluorescence Microscopy
HaCat human keratinocytes (Boukamp et al., 1988) were provided by
W.W. Franke (German Cancer Research Center, Heidelberg, Germany).
Transfection of human epidermoid carcinoma A-431 cells (CRL1555;
American Type Culture Collection, Rockville, MD) and selection,
growth, and immunofluorescence microscopy were done as described
(Chitaev et al., 1996
). The following mouse monoclonal antibodies were
used: anti-plakoglobin (clone 11E4; Zymed Laboratories, San Francisco,
CA); anti-desmoglein (clone 3.10; provided by W.W. Franke); anti-myc
(clone 9E10; provided by R. Kopan, Washington University, St. Louis,
MO); rabbit anti-myc antibody (Santa Cruz Biotechnology, Santa Cruz,
CA); anti-flag (Sigma Chemical Co.), and anti-
-catenin, anti-E-cadherin
(mAbs C20820 and C37020), anti-
-catenin, and anti-p120 (Transduction
Laboratories). In all cases, anti-E-cadherin antibody C20820 was used except where indicated.
Immunoprecipitation and Sedimentation Analysis
For most immunoprecipitation experiments, 2 × 106 cells were cultured in
10-cm tissue culture dishes at 37°C for ~72 h. In coculture experiments, 6 × 106 cells producing myc- and flag-tagged forms of E-cadherin mixed in a
ratio 1:1 were cultured in a 10-cm dish for 24 h. The confluent monolayer
(~107 cells) was then washed with PBS and extracted in 1.5 ml of lysis buffer (50 mM Tris-HCl, pH 7.4, 150 mM NaCl, 1 mM DTT, 20 µM
p-APMSF, 2 mM EDTA, and 1% NP-40) for 10 min. After clarification in
a microfuge (model 5415C; Eppendorf Scientific, Inc., Hamburg, Germany) for 10 min at 14,000 rpm, the lysates were immunoprecipitated for
1.5 h at 4°C in the presence of specific antibody (~1 µg per sample). The
antigene-IgG complexes were precipitated with sequential incubation
with protein A-Sepharose as described previously (Chitaev et al., 1996).
For the E-cadherin immunodepletion experiments, cell lysates were incubated with 5 µg of anti-E-cadherin (clones C37020 or C20820) or anti-Dsg
3.10 monoclonal antibodies. Then the antibodies were collected by two
rounds of anti-mouse IgG-agarose (Sigma Chemical Co.) chromatography. After repeating this step once (second round of immunodepletion),
the lysates were immunoprecipitated by anti-plakoglobin antibody as described above. For sucrose gradient centrifugation, confluent monolayer
cells from three 10-cm dishes, obtained as described above, were washed
with PBS and lysed with 2 ml of lysis buffer. For metabolic labeling experiments, cells were cultivated in the presence of [35S]methionine, 50 µCi/ml
for 16 h. Lysates (1 ml), precleaned by centrifugation (model TL-100;
Beckman Instrs., Inc., Palo Alto, CA) at 100,000 g for 1 h, were loaded on
top of a 12-ml linear 5-20% (wt/wt) sucrose gradient prepared in lysis
buffer. In some experiments, either 10 mM EGTA was added into gradients or EDTA was replaced with 1 mM CaCl2. Gradients, centrifuged at
200,000 g for 17 h in a rotor (model SW40Ti; Beckman Instrs., Inc., Palo Alto, CA) at 4°C, were fractionated from bottom to top into 12 fractions
(1 ml each), and then analyzed by coimmunoprecipitation. 50-µl aliquots
of each gradient fraction before immunoprecipitation were mixed with
concentrated (5×) SDS-PAGE loading buffer and analyzed by SDS-PAGE (Laemmli, 1970
) and immunoblotting. 5 µl of each fraction was
loaded. The following protein standards of known S values were centrifuged on replicate gradients: BSA, 4.5 S; IgG, 7.5 S; catalase, 11.35 S, apoferritin, 17 S.
Biotinylation of Cell Surface Proteins
The cells of three 10-cm dishes reaching near confluent growth were washed with ice-cold PBS containing 0.5 mM CaCl2 (PBS-C). Each plate was incubated at 4°C with 7 ml of 0.5 mg/ml of sulfo-NHS-LC-biotin (Pierce Chemical Co., Rockford, IL) in PBS-C for 1 h. The reaction was quenched by washing the cells with 1 M Tris/100 mM glycine buffer, pH 7.5. In some experiments, cells were dissociated into a single cell suspension by 5 min of treatment with 10 mM EGTA in PBS at 37°C after biotinylation. Then cells were lysed in lysis buffer and analyzed by sucrose gradient centrifugation and coimmunoprecipitation assays as described above. Biotinylated proteins were visualized with streptavidin-HRP conjugate (Pierce Chemical Co.) in conjunction with enhanced chemiluminescence (Boehringer Mannheim, Indianapolis, IN).
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Results |
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Lateral Dimers of E-cadherin Are Exposed on the Surface of Epithelial Cells
The cytoplasmic domain of E-cadherin binds to either
-catenin or plakoglobin (Butz and Kemler, 1994
; Hinck et
al., 1994
) that in turn, interacts directly with
-catenin (Jou et
al., 1995
). This gives rise to two distinct E-cadherin-catenin complexes, E-cadherin-
-catenin-
-catenin and E-cadherin-plakoglobin-
-catenin. The presence of a plakoglobin-
-catenin complex may indicate the assembly of these
conventional cadherin-catenin complexes into higher order structures. To test this hypothesis, we subjected Triton
X-100-soluble proteins from A-431 or HaCat cells to sucrose gradient fractionation followed by immunoprecipitation with anti-plakoglobin (Fig. 1 a) or anti-
-catenin
(data not shown) mAbs. Both types of experiments
showed that the conventional E-cadherin-catenin complexes sedimented at ~9 S, in agreement with published
results (Nelson et al., 1990
; Ozawa and Kemler, 1992
;
Hinck et al., 1995). However, the plakoglobin-
-catenin
complex separated into a distinct peak, sedimenting at 13 S. Both complexes were stable upon recentrifugation (Fig.
1, b and c), showing that the 9 S complex does not associate into a 13 S complex during in vitro manipulation. To
determine whether E-cadherin is part of the
-catenin-
plakoglobin complex, the 13 S fraction from metabolically
labeled proteins of A-431 cells was immunoprecipitated
with either anti-E-cadherin or anti-plakoglobin mAbs.
Immunoprecipitates were found to contain an identical set of proteins, E-cadherin, plakoglobin and
- and
-catenins
(Fig. 2 a). Furthermore, depletion of the 13 S fraction with
any of two anti-E-cadherin mAbs used in this work before
anti-plakoglobin immunoprecipitation strongly reduced
-catenin coimmunoprecipitation. Depletion with mAb
against desmoglein, that is desmosome-specific cadherin
of the A-431 cells, had no effect (Fig. 2 b). This suggests that the E-cadherin found in the 13 S fraction is complexed with plakoglobin and
-catenin. The plakoglobin-
-catenin complex detectable after E-cadherin immunodepletion is likely to contain P-cadherin, another classic
cadherin of A-431 cells.
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To show that the formation of this complex requires
dimerization of E-cadherin, we expressed in A-431 cells
human E-cadherin containing a 19-amino acid (aa)1
(His773-Leu791) long internal deletion in the cytoplasmic
domain and COOH-terminal 6× myc epitope (Ec1M, see
Fig. 3 a for details). As demonstrated by Western blotting
(Fig. 3 b), this deletion completely abolished binding of
E-cadherin to mAb C20820. Thus, cells stably transfected with the Ec1M DNA construct produce two forms of
E-cadherin that could be specifically recognized by mAb
C20820 (endogenous form) and by mAb against the myc
epitope (Ec1M form). Only cell subclones producing
Ec1M at the level similar to the level of endogenous E-cadherin, as estimated by immunoblotting of the total
lysates of the selected clones with C37020 antibody recognizing both E-cadherin forms (data not shown), were
studied. Double immunofluorescent microscopy of the
Ec1M-producing cells using rabbit anti-myc serum and
anti-E-cadherin mAb C20820 showed that the recombinant protein, despite the presence of this deletion, was incorporated efficiently into intercellular junctions (see Fig.
6). Western blot analysis of the immunoprecipitates obtained with anti-myc antibody showed that Ec1M, like
endogenous E-cadherin, coimmunoprecipitated plakoglobin, -catenin,
-catenin, and p120 (Fig. 4). Both endogenous and mutated E-cadherins have the same sedimentation properties (Fig. 3 c and not shown). Thus, the
His773-Leu791 deletion and addition of the 6× myc tag does
not influence the subcellular localization, sedimentation
properties, and association with catenins of E-cadherin.
These results allowed us to study dimerization of E-cadherin using the immunoprecipitation assay. Sucrose gradient sedimentation of Triton X-100-soluble proteins of the
A-431 cells expressing Ec1M and subsequent immunoprecipitation of the obtained fractions with anti-myc (Fig. 3 b)
or C20820 (data not shown) antibodies showed that the 13 S,
but not the 9 S complex, incorporates both endogenous
E-cadherin and Ec1M. Furthermore, biotinylation of the
cell surface proteins from these cells before lysis and after
sucrose gradient fractionation and anti-myc (data not
shown) or mAb C20820 (Fig. 3 c) immunoprecipitation,
clearly showed that the E-cadherin present in both 9 S and
13 S complexes is exposed on the cell surface.
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Experiments described above demonstrate that 13 S and
9 S E-cadherin complexes consist of the same proteins,
E-cadherin, - and
-catenins, and plakoglobin, suggesting
that the 13 S complex is a heterodimer of the E-cadherin-
-catenin-
-catenin and E-cadherin-plakoglobin-
-catenin (9 S) complexes. To determine whether the E-cadherin
found in the 13 S complex originates from the same or
from two opposing cells, the surface proteins of Ec1M-expressing cells were biotinylated and the cells dissociated
into a single cell suspension using 10 mM EGTA before lysis. The E-cadherin/Ec1M composition of the 13 S complex was not affected by complete dissociation of the cells
(Fig. 3 c). This shows that at least a significant portion of
the 13 S complex consists of E-cadherin molecules derived
from the same cell. Taken together, these data demonstrate a presence on the cell surface of the E-cadherin
complex in which both E-cadherin molecules are aligned
in parallel orientation.
The Extracellular EI Domain, But Not Binding to Catenins or p120, Is Required for Lateral E-cadherin Dimerization
Next, we examined whether binding to cytosolic proteins is
essential for lateral association of Ec1M with endogenous
E-cadherin. The truncated version of Ec1M, the Ec1(772-
882)M mutant (refer to Fig. 3 a and Fig. 4 for details), lacking the catenin-binding domain was expressed in A-431
cells. In agreement with the previous data (Nagafuchi and
Takeichi, 1988
; Ozawa et al., 1990b
), immunofluorescent microscopy and degradation of this mutant by trypsin treatment of the intact cells indicated that despite deletion of the
catenin-binding domain, the Ec1
(772-882)M protein was
transported to the cell surface. Results presented in Fig. 4
show that this mutant associates efficiently with endogenous E-cadherin. Besides catenins, in agreement with previous observations (Reynolds et al., 1994
; Shibamoto et al.,
1995
), minor fractions of the 9 S and 13 S E-cadherin-
catenins complexes were found to be associated with the
tyrosine kinase substrate p120 (refer to Fig. 1 a and Fig. 4 a).
Deletion of the catenin-binding domain in the Ec1
(772-
882)M mutant did not affect association with p120 (Fig. 4 a),
whereas it was completely abolished by a deletion of an additional 24-aa residues from the COOH terminus of the
Ec1
(772-882)M protein (Fig. 4 a). The resulting deletion mutant Ec1
(748-882)M was unable to bind p120 but
formed hybrid complexes with endogenous E-cadherin
(Fig. 4, a and b). As expected, the mobility of the hybrid
complex in a sucrose gradient shifted from fraction 6 to 7 due to the absence of the catenin-binding site in the mutant.
This complex was not affected by EGTA-induced dissociation of the cells. These experiments show that lateral dimerization of E-cadherin is mediated by its extracellular domain and does not depend on an interaction with the
cytoplasmic proteins p120, plakoglobin, and catenins.
X-ray crystallographic analysis (Shapiro et al., 1995; Nagar
et al., 1996
) showed that the extracellular domain of cadherin forms homodimers. Shapiro et al. (1995)
suggested
that the side chain of Trp156 of each cadherin molecule protrudes into the hydrophobic core of the neighbor molecule.
In the second model, the lateral dimers are stabilized by mutually coordinating calcium ions (Nagar et al., 1996
). Both
models are consistent with our observation that deletion of
the extracellular cadherin-like repeats 1-3 completely abolished association of the resulting Ec1
(159-536)M with
endogenous E-cadherin (data not shown). High stability of
the 13 S complex in 10 mM EGTA does not support the
role of Ca2+ in lateral dimerization. To determine whether
the Trp156 residue is required for E-cadherin dimerization,
we constructed an Ec1WVM combinatorial mutant in
which Trp156 and a neighbor residue, Val157, were substituted for Ala and Gly, respectively (refer to Fig. 3 a). In
A-431 cells, this mutant was translocated to the cell surface (data not shown) and formed a conventional 9 S trimer, but not the 13 S complex (Fig. 4 a). Additionally, the
Ec1WVM mutant and the other extracellular mutant
Ec1
(159-536)M, induced a strong dominant-negative effect on cell-cell adhesion (Fig. 4, c and d). A similar effect
has been described previously for different cadherin mutants lacking the extracellular region (Kintner, 1992
; Fujimori and Takeichi, 1993
). Because this phenotypic effect may abolish lateral E-cadherin association indirectly, we
determined whether these cells contain the 13S plakoglobin/
-catenin complex incorporating endogenous E-cadherin. This was done by analyzing the association between
plakoglobin and
-catenin using anti-plakoglobin (or anti-
-catenin) coimmunoprecipitation assays as described above. The data showed that the amount and sedimentation
properties of the 13 S complex were unchanged in control
and in transfected cells (data not shown), suggesting that a
failure of the Ec1WVM mutant to interact with endogenous
E-cadherin was not caused by a dominant-negative effect.
Thus, our data imply that lateral interaction between two
E-cadherin molecules in the 13S complex is mediated by the
mechanism proposed by Shapiro et al. (1995)
.
Adhesive, Head to Head, and Not Lateral E-cadherin Interaction Requires Catenins and Calcium
The data presented provide clear evidence that the lateral
dimerization of the E-cadherin is independent of calcium
and catenins. In contrast, homophilic cadherin-mediated
cell-cell adhesion strictly depends on both these factors,
suggesting that catenin and calcium may directly control
adhesive, but not lateral association between cadherins. Our
experiments with Ec1M protein, however, failed to demonstrate any multicadherin complexes other than lateral E-cadherin-catenin hexamers. The adhesive intercadherin
association, however, could be hidden in the experiments
described above if adhesive and lateral E-cadherin complexes have the same compositions and, hence, similar sedimentation properties. To test for the formation of adhesive
complexes in which E-cadherin-catenin complexes are arranged in antiparallel orientations, we applied an approach successfully used in our recent experiments with desmosomal cadherins (Chitaev and Troyanovsky, 1997). A-431
cells expressing Ec1M were cocultured overnight with A-431
cells stably producing the Ec1F form of E-cadherin. The latter protein contained the same internal deletion as Ec1M
and was selectively tagged by flag, but not the myc epitope.
In this coculture system, specific coimmunoprecipitation of Ec1F with anti-myc antibody would indicate the adhesive association between two forms of E-cadherin, whereas
the presence of endogenous E-cadherin in the same immunoprecipitates, assessed by mAb C20820, would show both
lateral and adhesive types of E-cadherin complexes.
Sedimentation-immunoprecipitation experiments with the total lysates obtained from such cocultures demonstrated that in the 13 S fractions anti-myc antibody did coimmunoprecipitate both flag-tagged and endogenous E-cadherin (Fig. 5). To show that the association between flag- and myc-tagged forms of E-cadherin depends on the integrity of cell-cell contacts, the cocultured cells were incubated for 10 min in 10 mM EGTA at 37°C before lysis in the regular lysis buffer. Complete disappearance of Ec1F, but not endogenous E-cadherin, in the anti-myc immunoprecipitates after EGTA treatment (Fig. 5 b, lanes 1 and 2) showed that the 13 S fraction contained two distinct lateral and adhesive E-cadherin complexes. To study whether reestablishment of the cell-cell contacts is accompanied by restoration of adhesive E-cadherin complexes, the cocultured cells, after incubation in 10 mM EGTA at 37°C, were further cultivated for the next 30 min either in low calcium or in normal medium (Fig. 5 b, lanes 3 and 4). The data show that the normal medium completely restored the amount of adhesive dimers (Ec1M-Ec1F complexes), whereas only Ec1M-E-cadherin complexes were detected in low calcium medium. Surprisingly, depletion of the calcium ions by EGTA did not reduce the amount of the E-cadherin-Ec1M complexes, which is a sum of the lateral and adhesive complexes (Fig. 5 and refer to Fig. 3). It can be suggested that the removal of extracellular calcium, while causing dissociation of the adhesive complexes, might increase the solubility of the lateral complexes which would account for the unchanged amount of the total complexes detected.
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To further evaluate the function of calcium ions in adhesive E-cadherin interactions, two additional experiments
were performed. First, the cocultured cells were incubated
before lysis for 10 min with EGTA at 4°C. At this temperature, in agreement with published observations (Citi,
1992), EGTA did not affect cell-cell junctions. In the second experiment, 10 mM EGTA was added to the lysis
buffer. In this case, the cells were not incubated with
EGTA before lysis. Surprisingly, we found that in both
these conditions EGTA did not decrease the adhesive association between flag- and myc-tagged forms of cadherins
(Fig. 5 b, lane 5 and data not shown). Taken together,
these data strongly suggest that calcium ions do not directly participate in the formation of the structure of the adhesive interface between two E-cadherin molecules.
This is consistent with the crystallography model reported
by Shapiro at al. (1995). Our experiments, however, did
not exclude the possibility that calcium might be important for one of the steps leading to the formation of adhesive dimers. To test this assumption, a new Ec1M mutant,
Ec1QNM, in which residues Gln255 and Asn256 were replaced with two alanines, was constructed. According to X-ray analysis, the replaced amino acids participate in coordination of two of the three Ca2+ ions filling the cleft between the ECI and ECII domains of E-cadherin (Nagar
et al., 1996
). Furthermore, it was shown that ablation of
one of these sites blocked E-cadherin cell-cell adhesion
activity (Ozawa et al., 1990a
). We found that the Ec1QNM
mutant upon expression in A-431 cells, similar to the
Ec1WVM mutant described above, was delivered to the
cell surface and induced a severe dominant-negative effect
on cell-cell adhesion (Fig. 6). This mutant normally associated with endogenous E-cadherin, but not with Ec1F (Fig.
5 b, lane 7), suggesting that defects in the Ca2+-binding
sites, while unable to change lateral dimerization, affect the adhesion interaction between two E-cadherin molecules. However, we could not discard the possibility that
the absence of such an interaction is caused indirectly by
the dominant-negative effect of the Ec1QNM mutant on the
cellular phenotype. Although additional experiments are
needed to completely understand the role of calcium in
cadherin-mediated adhesion, our data imply that binding
of calcium ions to cadherins is important for the formation
of adhesive dimers, that become independent of calcium
after their formation.
Finally, we determined whether mutations constructed for the characterization of lateral E-cadherin dimerization abolish the adhesive cadherin interaction. For this, we cocultivated the cells expressing these mutants with Ec1F-producing cells as described above. Anti-myc immunoprecipitation experiments presented in Fig. 5 b clearly show that the adhesive Ec1M-Ec1F association was completely abolished either by deletion of the catenin-binding region or by Trp156Ala/Val157Gly replacement (Fig. 5 b, lanes 6 and 8, respectively). The same factors, catenin and calcium, are therefore required for E-cadherin to form adhesive dimers and to establish cell-cell adhesion. This strongly suggests that the revealed dimers are structural elements of cadherin-mediated cell-cell adhesion.
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Discussion |
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---|
It is well established that the transmembrane protein E-cadherin forms complexes with intracellular -catenin (or plakoglobin) and with
-catenin (in this paper they are designated conventional E-cadherin-catenin complexes). This
association is absolutely required for E-cadherin to mediate intercellular adhesion (Nagafuchi and Takeichi, 1988
;
Ozawa et al., 1990b
). The exact role of catenins in this process is still unknown. It was also suggested (Shapiro et al.,
1995
; Brieher et al., 1996
; Nagar et al., 1996
; Tomschy et
al., 1996
), although never shown directly, that E-cadherin may form lateral dimers on the cell surface. These lateral
complexes, in which two E-cadherin molecules are aligned
in parallel orientation, were proposed to participate, in
turn, in the antiparallel interactions resulting in cell-cell
adhesion. The structural basis of both adhesive and lateral
interactions is not clear. In the present investigation, we
analyzed intercadherin interactions using an immunoprecipitation approach. To trace such interactions, we expressed in A-431 cells producing endogenous E-cadherin
recombinant forms of the same protein tagged either by
myc or by flag epitopes. Our findings not only present
compelling evidence for two distinct lateral and adhesive
E-cadherin complexes, but also allows us to clarify their
structures.
First, we obtained a strong evidence that the conventional E-cadherin-catenin complexes may self-associate
on the cell surface through E-cadherin dimerization. Our
data strongly support the idea that this process is driven by
hydrophobic interactions between the extracellular EI domains of E-cadherin. This mechanism was previously proposed by Shapiro et al. (1995). As suggested by sedimentation analysis (refer to Figs. 1 and 3), only a relatively small
pool of E-cadherin is incorporated into the lateral E-cadherin complexes. The formation of these E-cadherin complexes is independent of interactions of E-cadherin with
cytoplasmic proteins, such as catenins or p120. The fact
that even the longest deletion within the intracellular
E-cadherin region did not abolish lateral dimerization suggests that cytoplasmic factors are unlikely to regulate
assembly of these dimers. The amount of the lateral complexes was also independent of cell-cell interactions, since
it was stable (a) upon EGTA treatment leading to separation of cells, (b) in cells cultivated up to 1 wk in low calcium medium preventing establishment of cell-cell contacts (data not shown), and (c) in the cells with strong
dominant-negative abnormalities in cell-cell adhesion
caused by Ec1QNM expression. These data imply that lateral E-cadherin dimerization is not triggered in response
to head to head interaction with a protein(s) extended
from the opposing cell surface. Thus, if the E-cadherin lateral complex is not formed spontaneously, its assembly is
regulated either by soluble (humoral) factor(s) or by
transmembrane protein(s) extended from the same cellular surface.
Interestingly, independence of E-cadherin dimerization
from catenins indicates that the cell surface may contain
dimers in which E-cadherin molecules are linked either to
the same or to different catenins (plakoglobin and -catenin). This possibility was supported by our experiments
(Chitaev et al., 1998
) with A-431 cells expressing myc-tagged versions of
-catenin or plakoglobin. In both cell
types, anti-myc coimmunoprecipitation shows that the 13 S complex may contain two
-catenin or two plakoglobin molecules. Diversity of the lateral E-cadherin complexes
might even be larger since some may also incorporate different isoforms of p120. It is not clear whether such variety
has any biological significance. In theory, E-cadherin
dimers associated with different sets of catenins may have
distinct signaling or adhesive properties.
The second type of inter-E-cadherin interaction detected in our work is an adhesive interaction leading to the
formation of antiparallel E-cadherin complexes. Our experiments did not allow us to evaluate the exact structure
of such complexes, since these and lateral complexes were
present in the same fractions of the sucrose gradient. On
the other hand, several observations strongly suggest that,
similar to lateral complexes, they consist of two conventional E-cadherin-catenin complexes, but arranged in an antiparallel fashion. First, both lateral and antiparallel
complexes have the same sedimentation value. Second, no
differences were detected in protein composition of anti-
E-cadherin (or anti--catenin) radioimmunoprecipitates
obtained from the 13 S fraction from cells exhibiting (control), and not exhibiting (EGTA-treated) antiparallel complex (data not shown). Finally, immunoblotting experiments failed to reveal association with 13 S E-cadherin
complex other possible E-cadherin/catenin-associated proteins, such as EGF-receptor,
-actinin, vinculin, or actin.
These observations indicate similar protein composition
of the lateral and antiparallel E-cadherin complexes, although we cannot exclude that some of the peripheral proteins dissociate from these complexes during their solubilization in Triton X-100. The most important and specific
feature of adhesive complexes is the requirement for their
assembly of the same factors, extracellular calcium and
catenins, necessary for cell-cell adhesion. Such similarities
strongly suggest that the revealed antiparallel complexes
are structural units of cadherin-mediated cell-cell adhesion and their clustering, via interaction with the actin cytoskeleton (Knudsen et al., 1995
; Rimm et al., 1995
), may
be a step in adherens junction assembly.
The critical question is whether adhesive and lateral
complexes are the consecutive steps of one process, or are
uninterrelated, and participate in distinct processes, such
as signaling and adhesion. Although additional experiments are needed to understand this question, there is evidence in favor of the first hypothesis. We show that the
Trp156Ala/Val157Gly substitution which, according to
Shapiro et al. (1995), leaves an intact adhesive interface, abolishing both lateral and adhesive association. The latter
association, however, could be specifically blocked by removal of the catenin- or calcium-binding sites. This suggests that the adhesive complex is derived from lateral
complexes. A similar scenario was suggested by Brieher
et al. (1996)
, who found that lateral dimers of the recombinant extracellular portion of C-cadherin, participate in adhesion much more efficiently than monomers. Examination of intra-E-cadherin interactions by chimeric ECAD-COMP molecules also supports this view (Tomschy et al.,
1996
). The obvious problem is, that the head to head association of two lateral complexes must result in a structure
containing at least four conventional E-cadherin-catenin complexes. Our attempts to reveal E-cadherin complexes
greater than 13 S using different centrifugation protocols
were unsuccessful. Thus, the mechanism of the assembly
of the adhesive complexes remains open. One interpretation of our results is that a hypothetical antiparallel complex consisting of the four conventional E-cadherin-catenin units is very unstable. In normal cells this complex
dissociates at a high rate into two equal adhesive complexes characterized in our work. Alternatively, a lateral
E-cadherin complex may dissociate, giving rise to two activated E-cadherin-catenin complexes. They are subsequently used in adhesive associations. Importantly, both models would predict a special step, lateral-adhesive transition, in which two lateral E-cadherin dimers form two
antiparallel dimers. Catenins and calcium ions might be
functionally important for E-cadherin to proceed to this
transition. In the simplest model, catenins in response to
the lateral dimerization of E-cadherin would trigger a conformational change of each cadherin resulting in the activation of the E-cadherin adhesive site and concomitant dissociation of the lateral dimers. This model is consistent
with our data suggesting that calcium ions, which are
known to stabilize overall cadherin conformation (Pokutta
et al., 1996), could be involved only in formation, but not
in maintenance of the adhesive association.
In summary, our data present direct experimental evidence that E-cadherin may form lateral and adhesive complexes. They also show that interactions of E-cadherin with catenins and Ca2+ are essential for adhesive, but not for lateral intercadherin interactions. The major points for further investigation are the precise mechanisms leading to the formation of adhesive complexes and the role of catenins and other intracellular factors in this process.
![]() |
Footnotes |
---|
Received for publication 17 March 1998 and in revised form 30 June 1998.
This work has been supported in part by National Institutes of Health grant AR44016-03 and a research grant from the Dermatology Foundation.
![]() |
Abbreviation used in this paper |
---|
aa, amino acid(s).
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References |
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