Biochemical Characterization and Functional Analysis of Two Type II Classic Cadherins, Cadherin-6 and -14, and Comparison with E-cadherin*

Yutaka ShimoyamaDagger §, Hiroshi TakedaDagger , Shouko YoshiharaDagger , Masaki Kitajimaparallel , and Setsuo HirohashiDagger **

From the Dagger  Hirohashi Cell Configuration Project, Exploratory Research for Advanced Technology, Japan Science and Technology Corporation, Tsukuba Research Consortium, 5-9-4 Tokodai, Tsukuba 300-2635, the § Departments of Surgery and Clinical Research, National Okura Hospital, 2-10-1 Okura, Setagaya-ku, Tokyo 157-8535, the parallel  Department of Surgery, School of Medicine, Keio University, 35 Shinanomachi, Shinjuku-ku, Tokyo 160-8582, and the ** Pathology Division, National Cancer Center Research Institute, 5-1-1 Tsukiji, Chuo-ku, Tokyo 104-0045, Japan

    ABSTRACT
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Classic cadherins can be grouped based on their deduced primary structures. Among them the type I cadherins have been well characterized; however, little is known about non-type I cadherins. In this study we characterized two human type II cadherins, cadherin-6 and cadherin-14, using a cDNA transfection system. They were each detected as two bands electrophoretically, were expressed on the external cell surface at cell-cell contact sites, and were associated with caten- ins. Direct sequencing of the N-terminal amino acids showed that the two bands of cadherin-14 corresponded to precursor and mature forms, whereas the two bands of cadherin-6 both had the N-terminal sequence of the mature form. Unlike type I cadherins, both cadherin-6 and -14 were not protected from trypsin degradation by Ca2+. We evaluated their adhesive functions by a long term cell aggregation method. The results suggest that both cadherin-6 and -14 have cell-cell binding strengths virtually equivalent to that of E-cadherin and that their binding specificities are distinct from that of E-cadherin. Cadherin-6 and -14 interacted with each other in an incomplete manner. They have a QAI tripeptide in the first extracellular subdomain instead of the HAV motif that is characteristic of type I cadherins and is intimately involved in the adhesive function. The QAI tripeptide, however, appeared not to be involved in the adhesive functions of cadherin-6 and -14.

    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Cadherin was originally identified as a cell-cell adhesion molecule that functions in a Ca2+-dependent and homophilic manner and that is involved in various morphogenetic events during development (1). The first cadherins to be identified are known as the classic cadherins. In the last decade, numerous molecules that share the extracellular subdomain (EC)1 structure (cadherin repeat) of the classic cadherins have been discovered in both vertebrates and invertebrates, and they are now considered to constitute a large gene family, the cadherin superfamily. Besides the classic cadherins this family includes truncated type cadherins, desmosomal cadherins, protocadherins and protocadherin-related proteins, and HPT/LI-cadherins (2). The biological functions of most of these non-classic cadherins remain elusive.

Classic cadherins share a common primary structure that consists of a signal peptide and a prosequence, which are both removed by intracellular proteolytic processing, five cadherin repeats, a transmembrane domain, and a highly conserved cytoplasmic domain, which is essential for association with catenins, the ensuing linkage to the cytoskeleton, and full functioning as a Ca2+-dependent cell-cell adhesion molecule (3-5). Full cDNA cloning of 11 human classic cadherin molecules has been accomplished so far as follows: E-, N-, and P-cadherin, cadherin-4 (R-cadherin), -5, -6, -8, -11 (OB-cadherin), -12, -14, and -15 (M-cadherin) (6-14). Suzuki (2) proposed that the classic cadherins were divided into two subgroups, type I and type II, on the basis of their overall sequence similarities and the conservation of several motifs and aromatic amino acid residues in their extracellular domains. The human classic cadherins E-, N-, and P-cadherin and cadherin-4 have been classified as type I, and cadherin-6, -8, -11, -12, and -14 are classified as type II. Although cadherin-5 and -15 (M-cadherin) have been proposed to be type II and I, respectively (2), we think that they do not clearly belong to either subgroup (14).

The type I classic cadherins, especially E- and N-cadherin, have been well characterized both functionally and structurally. By contrast, characterization of the non-type I classic cadherins has just begun, and it is still not clear whether they behave as do E- and N-cadherin. It has been suggested that some of them have weaker cell-cell binding strengths than the type I cadherins because they are expressed in loosely associated cells (15). In fact, Suzuki and colleagues (2, 16) reported that cadherin-5 and -8 appear to lack strong cell-cell adhesion activity. Some of the type II cadherins, however, were reported to mediate definite cell-cell adhesion (11, 17). Thus, the relation of the molecular characteristics and functions of these non-type I classic cadherins to their roles in various tissues is intriguing.

We recently cloned two novel human type II cadherins, cadherin-6 and -14 (12, 13). In the present study we analyzed the two molecules in detail using an L fibroblast cDNA transfection system, and we compared them with E-cadherin. Friedlander et al. (18) and Steinberg and Takeichi (19) showed that the expression level of a cadherin can influence cadherin-mediated cell sorting, suggesting that it is important to check the relative expression level of each cadherin. However, a method for quantifying the expression of individual cadherins on the cell surface has not been established, so it is difficult to compare their binding strengths precisely. In this context, we have paid particular attention to the expression level of beta -catenin protein by our cadherin transfectants in order to semi-quantify the expression of cadherins and to evaluate their binding strengths and specificities. In this report we describe and discuss the functional characteristics of cadherin-6 and -14 together with their biochemical properties.

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INTRODUCTION
EXPERIMENTAL PROCEDURES
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Expression Vector Construction and Transfection-- To express human cadherin-6 and -14 in mouse L fibroblasts, the expression vectors pBAT6H and pBAT14H were constructed by replacing the mouse E-cadherin cDNA of pBATEM2 (20) with cDNA fragments covering the entire open reading frames of cadherin-6 and -14, respectively. Transfection of the expression vectors into L cells was performed using LipofectAMINE reagent (Life Technologies, Inc.) together with pSTneoB, which carries the neomycin resistance gene (21), according to the manufacturer's instructions. The transfected cells were selected in Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% calf serum in the presence of 400 µg/ml G418 in a humidified atmosphere comprising 5% CO2, 95% air at 37 °C for about 2 weeks. Then, the G418-resistant colonies were isolated, screened for cadherin-6 and -14 expression and maintained under the same conditions. Mouse E-cadherin transfectants were also obtained using pBATEM2 together with pSTneoB or pMAM2-BSD (Kaken Pharma Co.) and used as controls. When pMAM2-BSD was used, clones of the transfected cells were maintained in the presence of 5 µg/ml blasticidin S hydrochloride (Kaken Pharma Co.) instead of G418. Mouse L fibroblasts (LTK-) were supplied by the Riken Gene Bank.

We also used a newly reconstructed expression vector, designated pBAX, to prepare cadherin expression vectors and establish cadherin transfectants. pBAX was constructed by replacing the promoter region of pcDNA3 (Invitrogen Corp.) with that of pBATEM2 and reconstructing the multicloning sites. pBAX with cadherin cDNAs induced the expression of cadherin proteins in L cells at similar levels to pBATEM2 and its derivatives (data not shown).

To analyze the proteolytic processing of cadherin-6 and the functional significance of the QAI tripeptide in the first EC (EC1) of cadherin-6 and -14, amino acid substitutions were introduced into cadherin-6 and -14 by site-directed mutagenesis using the QuikChange Site-directed Mutagenesis Kit (Stratagene). The mutant molecules were expressed in L cells as described above.

Antibodies-- To produce a cadherin-6-specific antibody we generated a cadherin-6 fusion protein. A cadherin-6 cDNA fragment corresponding to EC5, a region with low homology to the other classic cadherins (12-14), and containing KpnI and HindIII sites at the 5'- and 3'-ends, respectively, was amplified by polymerase chain reaction, digested with KpnI and HindIII, and ligated to a prokaryotic expression vector, pRSET B (Invitrogen Corp.) that had been cleaved with the same enzymes. The resultant plasmid was introduced into an Escherichia coli strain, BL21(DE3)pLysS (Novagen), and expression of the fusion protein was induced by 1 mM isopropyl-beta -D-thiogalactoside. The protein was purified from bacterial lysates using a metal affinity resin (Talon, CLONTECH). A polyclonal anti-cadherin-6 antibody was then raised by immunizing rabbits with the fusion protein and was affinity purified using the same protein. A polyclonal anti-cadherin-14 antibody was raised by immunizing rabbits with a synthetic peptide, corresponding to the 15 C-terminal amino acids, conjugated to keyhole limpet hemocyanin, and affinity purified using the same peptide.

An anti-beta -catenin monoclonal antibody (Transduction Laboratories) was used to detect beta -catenin by immunoblotting and to immunoprecipitate cadherin-catenin complexes.

Short Term Cell Aggregation-- Dispersed cell suspensions were obtained by treating cells with 10 mM Hepes-buffered Ca2+- and Mg2+-free Hanks' solution (HCMF) containing 0.01% trypsin (crystallized porcine pancreas; Sigma) and 5 mM CaCl2 at 37 °C for 15 min at 80 rpm. Then they were washed three times with HCMF and suspended at 105 cell particles/ml HCMF containing 1% bovine serum albumin. The cell suspensions were added to a 24-well plastic plate (0.5 ml/well; Ultra Low Cluster; Corning Costar Corp.) with or without 5 mM CaCl2, and the cell particles were allowed to aggregate at 37 °C for 60 min at 80 rpm.

Long Term Cell Aggregation-- Completely dispersed cell suspensions were obtained by treating the cells with phosphate-buffered saline containing 0.05% trypsin and 0.02% EDTA at 37 °C for 15 min. Then the cells were washed twice with DMEM supplemented with 10% calf serum and were resuspended in DMEM supplemented with 10% calf serum and 70 units/ml DNase I (Takara) at a cell density of 2 × 105 cells/ml. The cell suspensions were added to a 24-well plastic plate (105 cells in 0.5 ml per well; Ultra Low Cluster; Corning Costar Corp.) and allowed to aggregate at 37 °C for 48 h at 100 rpm in a humidified atmosphere comprising 5% CO2, 95% air. To examine the heterotypic interactions between the cadherin subclasses, mixed cell-type aggregation experiments were performed using two transfectant cell lines expressing different cadherins; one line was labeled with 40 µg/ml 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate (DiI; Molecular Probes) in DMEM supplemented with 10% calf serum for 1 h and the other was unlabeled. The cells were suspended as described above, and equal numbers of cells of the two cell lines (5 × 104 in 0.25 ml each) were mixed and allowed to aggregate for 12 h as described above.

Immunoblotting and Immunocytochemistry-- Immunoblot analysis was carried out as described previously (4) except that the antigens were detected using the ECL system (Amersham Pharmacia Biotech). To quantify the amount of beta -catenin protein in the cells, the density of each band of beta -catenin was determined by densitometry and normalized for those of the parent L cells and the LE-5 transfectant cell line, which expresses mouse E-cadherin at a high level.

L transfectants cultured on plastic dishes were fixed with 4% paraformaldehyde and 2% sucrose in 10 mM Hepes (pH 7.4), 150 mM NaCl, 2 mM CaCl2 (HNC, a buffer containing 10 mM Hepes (pH 7.4), 150 mM NaCl, 2 mM CaCl2) at 4 °C for 10 min and then with methanol at 4 °C for 30 min. The dishes were heated at 90 °C for 10 min in HNC buffer containing 1% 2-mercaptoethanol and then rinsed extensively with water and finally with HNC. After treatment with 5% bovine serum albumin in HNC for 1 h, the cells were incubated with the affinity purified anti-cadherin-6 or -14 antibody at 4 °C overnight. They were then incubated with biotinylated anti-rabbit IgG (Vector Laboratories) at room temperature for 1 h, followed by 1-h incubation with fluorescein isothiocyanate-conjugated streptavidin (Vector Laboratories). Finally, after extensive rinsing with HNC, they were mounted with Perma Fluor (Shandon Lipshaw) and examined with a Zeiss Axiophot microscope.

Other Biochemical Procedures-- Immunoprecipitation, N-terminal amino acid sequencing, and determination of the trypsin sensitivity was performed as described previously (14). Exposure of cadherin molecules on the surface of the transfected L cells was also examined as described previously (14).

The N-linked oligosaccharides of cadherin-6 were removed by enzymatic deglycosylation. L6-33 cells were lysed with 50 mM Tris-HCl (pH 8.6), 1% Nonidet P-40, 1 mM phenylmethylsulfonyl fluoride, 20 µg/ml leupeptin. The cell lysate was clarified by centrifugation, heated at 100 °C for 5 min, incubated with various amounts of glycopeptidase F (peptide:N-glycosidase F; Takara) at 37 °C for 18 h, and then analyzed by immunoblotting with the anti-cadherin-6 polyclonal antibody.

    RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Expression of Cadherin-6 and -14 by L Cells-- L cells, which are mouse lung fibroblasts deficient in cadherin activity (22), were transfected with pSTneoB and either pBAT6H or pBAT14H. Over 30 transfectant clones of each cadherin were isolated after G418 selection and screened for cadherin expression. Concomitantly, transfectant clones of cells transfected with pSTneoB, pBAX, or pMAM2-BSD, the control clones, were isolated; they were indistinguishable from the parent L cells based on the tests used in this study (data not shown).

The transfectant clones designated L6-33 and L14-4 showed the highest levels of cadherin-6 and -14 expression, respectively, in immunoblots (Fig. 1). Two bands of protein of approximately 125 and 120 kDa were labeled by the anti-cadherin-6 polyclonal antibody (Fig. 1A), and two bands of protein of approximately 112 and 105 kDa were labeled by the anti-cadherin-14 polyclonal antibody (Fig. 1B). As reported previously (23), these cadherin transfectants exhibited elevated levels of beta -catenin protein (Fig. 1C) as well as alpha -catenin protein (data not shown), suggesting that both cadherin-6 and -14 interact with catenins, form cadherin-catenin complexes, and stabilize catenins, as do other classic cadherins (24). The association of cadherin-6 and -14 molecules with catenins was confirmed by immunoprecipitation experiments using the anti-beta -catenin monoclonal antibody. The antibody precipitated cadherin-6 and -14 molecules, which showed the same mobilities and band patterns on sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) as in the immunoblotting samples (Fig. 1, A and B), as well as alpha - and beta -catenins (Fig. 2). To determine the difference between the two forms of cadherin-6 and -14, each band stained with Coomassie Blue was cut from the polyvinylidene difluoride (PVDF) membrane (Millipore), and the N-terminal amino acid sequence was determined.


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Fig. 1.   Immunoblot analysis of cadherin transfectants. Cell lysates of L, L6-33, L14-4, L6PRE-2, L6HAV-6, L14HAV-6, LE-1, and LE-5 cells (20 µg protein/lane) were separated by 7.5% SDS-PAGE and transferred to PVDF membranes. A, cadherin-6 was detected with an anti-cadherin-6 polyclonal antibody. The two main bands of cadherin-6 are indicated by arrows. The lower bands in the L6-33 sample probably indicate degradation of cadherin-6. B, cadherin-14 was detected with an anti-cadherin-14 polyclonal antibody. The two main bands of cadherin-14 are indicated by arrows. The lower bands in the L14-4 sample probably indicate degradation of cadherin-14. C, beta -catenin was detected with an anti-beta -catenin monoclonal antibody. The lower bands in the LE-5 sample probably indicate degradation of beta -catenin. Bars on the left indicate the mobilities of molecular mass markers (200, 116, and 97.4 kDa in A, 200, 116, 97.4, and 66.2 kDa in B, and 200, 116, 97.4, 66.2, and 45 kDa in C).


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Fig. 2.   Immunoprecipitation of cadherin-6 and -14 with an anti-beta -catenin monoclonal antibody. L6-33 or L14-4 cell lysate was incubated with normal mouse IgG (N) or the anti-beta -catenin monoclonal antibody (beta ). The precipitates were denatured, separated by 7.5% SDS-PAGE, transferred to a PVDF membrane, and stained with AuroDye Forte Kit (Amersham Pharmacia Biotech). The cadherin-6 and -14 and alpha - and beta -catenin bands are indicated by arrows and arrowheads, respectively. The faint bands below the beta -catenin bands are beta -catenin degradation products, which was confirmed by immunoblotting (data not shown), and the intense lower bands are derived from immunoglobulins. Bars on the left indicate the mobilities of molecular mass markers (200, 116, 97.4, 66.2, and 45 kDa).

The sequence of the larger (112 kDa) cadherin-14 molecule was Thr-Ala-His-His-Ser-Ser-Ile-Lys-Val-Met-Arg, indicating that it is a precursor form of cadherin-14 that is cleaved between Gly-24 and Thr-25 by signal peptidases. This site agrees with possible cleavage sites of eukaryotic signal peptides proposed by Nielsen et al. (25). The N-terminal sequence of the shorter cadherin-14 molecule (105 kDa) was Gly-Trp-Val-Trp-Asn-Gln-Phe-Phe-Val-Leu-Glu-Glu, indicating that it is a mature form of cadherin-14 that is cleaved just after a pair of basic amino acids (Lys-52, Arg-53) by endopeptidases. By contrast, the two cadherin-6 peptides (125 and 120 kDa) had the same N-terminal sequence, Ser-Trp-Met-Trp-Asn- Gln-Phe-Phe-Leu-Leu-Glu-Glu, indicating that they both correspond to a putative mature form of cadherin-6 (12) that is proteolytically processed.

We wondered whether one of the two cadherin-6 peptides was an N-terminally blocked non-mature form, and this result was due to contamination of this band by the mature form, because the two bands were contiguous (Figs. 1A and 2). We repeated the analysis and obtained the same result. Next we prepared a mutant cadherin-6 molecule with a single amino acid substitution of Arg-53 to Gly, which would not be cleaved to the mature form of cadherin-6 and which would correspond to a precursor form of cadherin-6. To do this we replaced an A with a G at nucleotide position 276, expressed the mutant in L cells, and compared the gene product with the two molecular forms of cadherin-6 by immunoblotting (Fig. 3). The immunoblot analysis showed that the mutant cadherin-6 expressed in an L cell transfectant clone, designated L6PRE-2, also resulted in two protein bands on SDS-PAGE, with higher molecular masses than the wild-type cadherin-6 molecule expressed by L6-33 cells. These findings show that the larger wild-type cadherin-6 is not a precursor form, unlike the larger cadherin-14 protein, and suggest that both bands of cadherin-6 were mature forms.


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Fig. 3.   Immunoblot analysis of wild-type and mutant cadherin-6. Cell lysates of L6-33, L6PRE-2, and L6HAV-6 cells were separated by 7.5% SDS-PAGE, transferred to PVDF membranes, and probed with an anti-cadherin-6 polyclonal antibody. The amount of protein in each lane was not adjusted in this blot. The lower bands in all the lanes probably indicate degradation of cadherin-6. Bars on the left indicate the mobilities of molecular mass markers (200, 116, 97.4, and 66.2 kDa).

We previously reported that the deduced cadherin-6 protein sequence contains five possible N-linked glycosylation sites (12). To examine the influence of glycosylation on the mobility of cadherin-6, N-linked oligosaccharides were removed enzymatically. Fig. 4 shows the N-deglycosylation effect of various concentrations of glycopeptidase F on cadherin-6; the molecular masses of the pair of cadherin-6 bands were reduced stepwise as the enzyme concentration increased; however, the two-band pattern never changed. We also used tunicamycin, an inhibitor of N-linked oligosaccharide synthesis, but the two-band pattern remained unchanged (data not shown).


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Fig. 4.   N-Deglycosylation effect of glycopeptidase F on cadherin-6. L6-33 cell lysate was treated with glycopeptidase F at 0 (lane 1), 0.005 (lane 2), 0.02 (lane 3), 0.05 (lane 4), 0.2 (lane 5), 0.5 (lane 6), 2.0 (lane 7), 5.0 (lane 8), and 50 milliunits/ml (lane 9) at 37 °C for 18 h and then analyzed by immunoblotting with an anti-cadherin-6 polyclonal antibody. Bars on the left indicate the mobilities of molecular mass markers (200, 116, and 97.4 kDa).

The subcellular distributions of cadherin-6 and -14 in the transfectant clones L6-33 and L14-4, respectively, were examined immunocytochemically (Fig. 5). As expected, both cadherin-6 and -14 were concentrated at cell-cell contact sites. Furthermore, exposure of cadherin-6 and -14 molecules on the external cell surface was confirmed by extracellular biotin labeling of the cadherins (Fig. 6). Unexpectedly, this experiment showed that not only the mature forms of cadherin-6 and -14 but also the precursor form of cadherin-14 were exposed on the cell surface.


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Fig. 5.   Immunocytochemical detection of cadherin-6 and -14. Cadherin-6 expressed in L6-33 and cadherin-14 expressed in L14-4 cells were detected by immunofluorescent staining with an anti-cadherin-6 polyclonal antibody and an anti-cadherin-14 polyclonal antibody, respectively. Both cadherins were concentrated at cell-cell contact sites. Scale bar, 100 µm.


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Fig. 6.   Exposure of cadherin-6 and -14 on cell surfaces. L6-33 and L14-4 cell membrane proteins were biotinylated extracellularly, immunoprecipitated with an anti-beta -catenin monoclonal antibody, separated by 7.5% SDS-PAGE, and electroblotted onto PVDF membranes. Then the immunoprecipitates were stained with AuroDye Forte Kit to detect all of the proteins (A) or with diaminobenzidine using the avidin-biotin-peroxidase complex (Elite ABC; Vector Laboratories) to detect proteins exposed on the cell surface (B). The cadherin-6, cadherin-14, alpha -catenin, and beta -catenin bands are indicated by arrowheads. Both forms of cadherin-6 and -14 were biotinylated, indicating that all four proteins were exposed on the external cell surface. Note that the catenins were not biotinylated, demonstrating the reliability of this experiment. Bars on the left indicate the mobilities of molecular mass markers (200, 116, and 97.4 kDa).

Cell-Cell Binding Activities and Biochemical Properties of Cadherin-6 and -14-- The exposure of cadherin-6 and -14 at cell-cell contact sites, as shown in Figs. 5 and 6, suggests that these molecules function as intercellular connectors, as do type I cadherins. We first examined their cell-cell binding activities using a conventional method, the short term cell aggregation assay. We also examined the up-regulation of beta -catenin protein expression in L cells with introduced cadherins (Fig. 1C). Assuming that the different cadherins interact with beta -catenin and contribute to its preservation in a similar manner, the binding strengths of the cadherins can be compared using transfectants that express equal amounts of beta -catenin protein. Both the L6-33 and L14-4 cells, however, exhibited only weak Ca2+-dependent cell-cell aggregation in this assay system as compared with LE-1 cells and other E-cadherin transfectants (data not shown) that express almost the same amount of beta -catenin (Table I).

                              
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Table I
Short-term cell aggregation of cadherin transfectants
Cell suspensions obtained after treatment with trypsin in the presence of Ca2+ were plated into 24-well plastic plates without (Ca(-)) or with (Ca(+)) 5 mM CaCl2 in triplicate and allowed to aggregate at 37 °C for 60 min at 80 rpm. The extent of cell aggregation is represented by the aggregation index (n0-n60)/n0, where n60 and n0 are the mean total numbers of particles after incubation for 60 min and at the start of incubation, respectively. Values are the means of at least three separate experiments.

We recently reported that the susceptibility of cadherin-15 to trypsin digestion in the presence of Ca+ causes a low aggregation rate in the short term assay (14). We therefore examined the trypsin sensitivities of cadherin-6 and -14 (Fig. 7). Both molecular forms of cadherin-6 were digested by trypsin treatment, even in the presence of Ca2+, whereas most of the mature form of cadherin-14 was digested by trypsin but a small fragment remained regardless of the presence of Ca2+. The mature form of cadherin-14 appeared to be slightly more stable in the presence of Ca2+ than in the absence of Ca2+, and partially digested molecules were detected only in the presence of Ca2+. Interestingly, a fragment of the precursor form of cadherin-14 was detected after the trypsin treatment. These results suggest that the low Ca2+-dependent cell-cell aggregation rates described above were due to the digestion of cadherin-6 and -14 by trypsin and thus that the conventional aggregation assay cannot be used to evaluate the cell-cell adhesion activities of these cadherins correctly.


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Fig. 7.   Trypsin sensitivity of cadherin-6 and -14. L6-33 and L14-4 cells were treated with HCMF containing 5 mM CaCl2 (N), or 0.01% trypsin and 1 mM EGTA (TE), or 0.01% trypsin and 5 mM CaCl2 (TC) at 37 °C for 15 min and were analyzed by immunoblotting with an anti-cadherin-6 polyclonal antibody and an anti-cadherin-14 polyclonal antibody, respectively. Whole cell lysates derived from the same number of cells were loaded onto each lane. A possible precursor form of cadherin-14, which was reduced in molecular mass by trypsin treatment, was detected (arrow). A partially digested fragment of cadherin-14 was also detected (arrowhead). Bars on the left indicate the mobilities of molecular mass markers (200, 116, 97.4, and 66.2 kDa).

After treatment with trypsin and EDTA to destroy most of the E-cadherin, cadherin-6, and cadherin-14 molecules expressed by the transfected L cells, the expression levels of these cadherins returned to the initial levels within 3 h (data not shown). Therefore, we repeated the cell aggregation assay using a 48-h aggregation period to compare the cell-cell binding activity of each cadherin. The influence of trypsin pretreatment to disperse the cells was considered to be negligible in these assays. The results are shown in Fig. 8. After 48-h incubations L6-33 and L14-4 cells formed aggregates that were almost indistinguishable in both size and cell-cell adhesiveness from LE-1 aggregates, whereas virtually no parent L cell aggregation was observed under the same conditions (Fig. 8). Therefore, both cadherin-6 and -14 do function as cell-cell connectors. Taking account of the almost equivalent level of beta -catenin protein expressed in these three transfectant cell lines (Fig. 1 and Table I) and assuming that these lines express almost equivalent numbers of cadherin molecules per cell, these results suggest that the cell-cell binding strengths of these three cadherins are virtually the same. Our observations that LE-5 cells with a higher beta -catenin expression level (Fig. 1 and Table I) formed larger and tighter aggregates (Fig. 8) and that many transfectant lines that expressed beta -catenin at lower levels than L6-33, L14-4, and LE-1 cells formed smaller aggregates (data not shown) support the above idea. In addition, L6PRE-2 cells, which expressed a mutant cadherin-6 molecule corresponding to its precursor form (Fig. 3), did not show any significant aggregation (Fig. 8). This result indicates that, as has been demonstrated for E-cadherin (26), cadherin-6 requires the removal of the precursor segment by proteolytic processing for its cell-cell binding activity.


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Fig. 8.   Long term cell aggregation of cadherin transfectants. L (A), L6-33 (B), L14-4 (C), LE-1 (D), LE-5 (E), L6PRE-2 (F), L6HAV-6 (G), and L14HAV-6 (H) cells were trypsinized completely in the presence of EDTA to obtain single cells, which were suspended in DMEM supplemented with 10% calf serum and 70 units/ml DNase I. The cells (105 cells in 0.5 ml per well) were plated in a 24-well plastic plate and allowed to aggregate at 37 °C for 48 h at 100 rpm in a CO2 incubator. Then phase-contrast micrographs were taken. Scale bar, 200 µm.

We next performed mixed cell aggregation experiments to determine the cell-cell binding specificities of cadherin-6 and -14. First, L6-33 cells or L14-4 cells were mixed with L cells and allowed to aggregate; both the L6-33 cells and L14-4 cells formed aggregates that excluded the parent L cells (data not shown), indicating that cadherin-6 and -14 mediate cell-cell adhesion in a homophilic manner, as do other classic cadherins (1, 14). Next, one cell line was labeled with 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate (DiI) reagent, mixed with another unlabeled line, and allowed to aggregate for 12 h. Representative results are shown in Fig. 9. When DiI-labeled and unlabeled cells of the same cell line were mixed, randomly intermixed aggregates were formed (Fig. 9, A and B). When LE-1 cells were mixed with L6-33 or L14-4 cells, the LE-1 cells aggregated separately from the L6-33 or L14-4 cells, and chimeric aggregates were not found (Fig. 9, C and D). Interestingly, when L6-33 and L14-4 cells were mixed, chimeric aggregates composed of clusters of each cell type were formed (Fig. 9, E and F). We performed this set of experiments repeatedly and always observed similarly intermixed aggregates. These findings indicate that cadherin-6 and -14 possess binding specificities distinct from that of E-cadherin and that they partially interact with each other.


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Fig. 9.   Mixed cell aggregation of cadherin transfectants. DiI-labeled L6-33 cells (5 × 104) were mixed with an equal number of unlabeled L6-33 (A and B), LE-1 (C and D), or L14-4 cells (E and F) in DMEM supplemented with 10% calf serum and 70 units/ml DNase I and were allowed to aggregate, as described in the legend to Fig. 8, for 12 h. Phase-contrast (A, C, and E) and fluorescence (B, D, and F) micrographs of the same fields are shown. DiI-labeled and unlabeled L6-33 cells formed randomly mixed aggregates (A and B). When DiI-labeled L6-33 cells were mixed with unlabeled LE-1 cells, mixed cell aggregates were not seen (C and D), whereas L6-33 and L14-4 cells formed chimeric aggregates composed of clusters of each cell type (E and F). Scale bar, 100 µm.

The HAV motif in the EC1 of type I classic cadherins is intimately involved in their adhesive functions (27-29), whereas the HAV motif is replaced by a QAI tripeptide in cadherin-6 and in cadherin-14. To determine the significance of the QAI tripeptide to the adhesive functions of cadherin-6 and -14, mutant cadherin-6 and -14 cDNAs that encoded HAV instead of the QAI tripeptide were constructed by replacing the A at nucleotide positions 507 and 511 (12) with C and G, respectively, in cadherin-6 and by replacing the A at nucleotide positions 700 and 704 (13) with C and G, respectively, in cadherin-14. These mutated cadherin-6 and -14 cDNAs were introduced into L cells using the pBAX expression vector, and transfectant lines stably expressing each mutant molecule were cloned. The L6HAV-6 and L14HAV-6 lines, which showed the highest expression of the mutant cadherin-6 and -14 molecules, respectively, were used for further analyses. These mutant molecules appeared to be indistinguishable from the respective wild-type molecules except that the mutant cadherin-6 molecule migrated more slowly than the wild-type cadherin-6 on SDS-PAGE (Fig. 3). The mutant cadherin-14 molecule showed almost the same mobility as that of the wild-type cadherin-14 on SDS-PAGE (data not shown). Compared with L6-33 and L14-4 cells, L6HAV-6 and L14HAV-6 cells showed lower expression of beta -catenin protein (Fig. 1 and Table I), and they formed smaller aggregates in long term cell aggregation experiments (Fig. 8).

L6HAV-6 and L14HAV-6 cells were tested in mixed cell aggregation experiments to examine the effect of the conversion of the QAI tripeptide to HAV on the adhesive functions of cadherin-6 and cadherin-14. Representative results are shown in Fig. 10, and the interactions between different cadherins are summarized in Table II. L6HAV-6 and L14HAV-6 cells formed almost randomly mixed aggregates with L6-33 and L14-4 cells, respectively (Fig. 10, A, B, E, and F). When L6HAV-6 and L14-4 cells, as well as L14HAV-6 and L6-33 cells, were mixed chimeric aggregates composed of clusters of each cell type were formed (Fig. 10, C, D, G, and H). Moreover, L6HAV-6 and L14HAV-6 cells never formed chimeric aggregates with LE-1 cells (Table II). Thus, the conversion of QAI to HAV did not appear to affect the binding specificities of cadherin-6 and -14 in this series of experiments. We also examined the effects of synthetic peptides, including the QAI tripeptide (LRAQAINRRT for cadherin-6 and LHAQAIDRRT for cadherin-14), on cell aggregation of cadherin-6 and cadherin-14 transfectants, but we did not observe any inhibitory effects (data not shown).


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Fig. 10.   Effect of a mutation of QAI to HAV in cadherin-6 and -14 on mixed cell aggregation. Equal numbers (5 × 104) of DiI-labeled L6HAV-6 and unlabeled L6-33 cells (A and B), DiI-labeled L6HAV-6 and unlabeled L14-4 cells (C and D), DiI-labeled L14HAV-6 and unlabeled L14-4 cells (E and F), or DiI-labeled L14HAV-6 and unlabeled L6-33 cells (G and H) were mixed and allowed to aggregate as in Fig. 9. Phase-contrast (A, C, E, and G) and fluorescence (B, D, F, and H) micrographs of the same fields are shown. Scale bar, 100 µm.

                              
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Table II
Summary of interactions between cadherins
This table is based on the results of mixed cell aggregation experiments.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Many members of the cadherin superfamily have been discovered in the last decade; over 20 classic cadherins have been identified in various vertebrates. To our knowledge, in humans 11 classic cadherins have been characterized so far by full cDNA cloning and sequencing. The classic cadherins can be divided into subtypes (type I, type II, and others) on the basis of their deduced amino acid sequences (2, 14). Among the classic cadherins, E- and N-cadherin, both of which are type I cadherins, have been investigated most thoroughly and have been well characterized; however, little is known about the other, especially the non-type I, cadherins. We therefore planned to analyze the molecular nature of cadherin-6 and -14, both of which are classified as type II classic cadherins.

Cadherin-6 and -14 cDNAs were introduced into mouse L fibroblasts, and transfectant clones stably expressing each cadherin were isolated. Immunoprecipitation and immunoblot experiments showed that these cadherins interacted with and stabilized catenins, as does E-cadherin. On SDS-PAGE cadherin-6 and -14 were seen as two bands, 125 and 120 kDa, and 112 and 105 kDa proteins, respectively. It is widely thought that transcribed cadherin molecules are cleaved by signal peptidases on the endoplasmic reticulum membranes and that the resultant precursor forms undergo further proteolytic processing by endoproteases to generate the functional mature forms (26). Indeed, a faint band is often observed just above the main band of a cadherin on immunoblotting, which may correspond to the precursor form (30). Here, we demonstrated that the larger of the two cadherin-14 proteins seen on SDS-PAGE was indeed a precursor that had been cleaved just after the signal peptide and that at least part of the precursor was exposed on the cell surface similar to the mature form. The significance of the cadherin-14 precursor on the cell surface remains unclear at present. We also detected two cadherin-6-positive bands; however, direct sequencing of each protein showed that they had the same N terminus as the putative mature form of cadherin-6; both were expressed on the external cell surface, and they had similar trypsin sensitivities and detergent solubilities.2 Interestingly, cadherin-6 expressed in various human cell lines also shows the same two-band pattern.2

The phosphorylation of a protein often alters its mobility on SDS-PAGE. We therefore examined, by potato acid phosphatase treatment (31) and immunoblot analysis using antibodies against phosphoamino acid residues (32), whether the two forms of cadherin-6 are phosphorylated and non-phosphorylated forms of the mature cadherin-6 protein, but phosphorylation of cadherin-6 does not seem to alter its electrophoretic mobility.2 It is also unlikely that there is post-translational modification of the C-terminal region, because anti-pan cadherin rabbit serum (Sigma) raised against the C-terminal sequence of chicken N-cadherin detects both bands on immunoblots.2

It is well known that cadherins undergo sugar modifications (33, 34) and that cadherin-6 has five consensus sites for N-linked glycosylation (12). Therefore, we suspected that the two molecular forms of cadherin-6 might represent different stages of glycosylation. However, the two bands were not replaced by a single band after treatment with glycopeptidase F or tunicamycin, although these experiments could not rule out the above possibility completely. Note that in the N-deglycosylation experiment using glycopeptidase F, the relative molecular mass of cadherin-6 became smaller in a stepwise manner as the enzyme concentration increased (Fig. 4). For example, the upper band of cadherin-6 is clearly seen in the 0.5 milliunit/ml glycopeptidase F sample, but this band becomes faint at 2 milliunits/ml glycopeptidase F and is absent at 5 milliunits/ml glycopeptidase F; the cadherin-6 molecule corresponding to the upper band at 0.5 milliunit/ml glycopeptidase F appears to be migrating at the same rate as the lower band with the advance of deglycosylation (Fig. 4). If this is the case, the difference between the two molecular forms of mature cadherin-6 may result from one N-linked oligosaccharide chain that is resistant to experimental deglycosylation. At present, this issue and the difference in adhesive function between the two forms remains to be resolved.

At an early stage of cadherin research the resistance of cadherin to trypsin degradation in the presence of Ca2+ was considered a hallmark of the cadherin family (1). However, the present study has demonstrated clearly that both cadherin-6 and -14 were not fully protected from trypsin by Ca2+. We reported recently that cadherin-15, a human homologue of mouse M-cadherin, is also sensitive to trypsin in the presence of Ca2+ (14) and Tanihara et al. (16) described similar trypsin sensitivity for cadherin-5. Thus, protection from trypsin degradation by Ca2+ may not be a common feature of cadherin family members, particularly for non-type I classic cadherins.

Cell-cell adhesion activities of cadherins have been evaluated mainly by short term cell aggregation assays, in which cells dispersed by trypsin treatment in the presence of Ca2+ were studied (35). However, we have found that this assay system does not always accurately evaluate the cell-cell adhesive functions of cadherins. Therefore, we used a long term cell aggregation assay in this study. Another important point to be considered when evaluating cadherin function is how individual cadherin molecules are quantified. Therefore, we measured the expression level of beta -catenin protein in the cadherin transfectants used in this study. We assumed that in the L fibroblast cDNA transfection system each classic cadherin subclass interacts with and stabilizes beta -catenin in a similar manner and that, therefore, the binding strength and specificity of each cadherin subclass can be compared using transfectants that express equal amounts of beta -catenin protein. Thus, we used cadherin-6, cadherin-14, and E-cadherin transfectants that expressed almost the same amount of beta -catenin protein to evaluate the adhesive functions of these cadherins. In the long term cell aggregation experiments, all of the transfectants formed aggregates that were similar in both size and cell-cell adhesiveness, suggesting that the cell-cell binding strengths of cadherin-6, cadherin-14, and E-cadherin are virtually equivalent. Moreover, the mixed cell aggregation experiments showed that both cadherin-6 and -14 had binding specificities distinct from that of E-cadherin. Interestingly, these experiments also showed that cadherin-6 and -14 can interact with each other in an incomplete manner. Similar heterophilic interactions between cadherins from the same species have been described for N-cadherin and R-cadherin (cadherin-4) (36, 37), chick B-cadherin and liver cell adhesion molecule (L-CAM) (38), and chick cadherin-6B and -7 (17). It is possible that heterophilic interactions between cadherins of different subclasses are responsible for the interaction of adjacent tissues in vivo, because in the mixed cell aggregation experiments referred to above chimeric aggregates composed of clusters of each cell type were observed, except for the combination of chick B-cadherin and L-CAM. Much more work is necessary, however, to elucidate the significance of these interactions.

It is widely accepted that the HAV tripeptide motif, which resides in EC1 of type I classic cadherins, and its flanking amino acids is intimately involved in the adhesive function and binding specificity (27-29). In non-type I classic cadherins, however, the HAV motif is replaced by other tripeptides (14), but it is not known whether these tripeptides are involved in the binding functions of the cadherins. Both cadherin-6 and -14 have a QAI tripeptide instead of the HAV motif (12, 13), prompting us to investigate whether the QAI motif is involved in the binding specificities of cadherin-6 and -14, especially the partial interaction between cadherin-6 and -14. We constructed mutant cadherin-6 and -14 molecules that had the HAV motif instead of QAI, but this mutation had no effect on the binding specificities of cadherin-6 and -14. We also examined the effects of synthetic peptides, including the QAI tripeptide, on cell aggregation of cadherin-6 and cadherin-14 transfectants, but they did not show any inhibitory effects. Thus, we did not observe any evidence that the QAI tripeptide and its flanking amino acids are involved in the adhesive functions of cadherin-6 and -14 and the region that is responsible for the adhesive functions of the non-type I classic cadherins remains to be identified. More detailed studies including structural analyses will provide answers to this question.

    ACKNOWLEDGEMENT

We thank Dr. M. Takeichi for providing the pBATEM2 and pSTneoB expression vectors.

    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: Dept. of Surgery, National Okura Hospital, 2-10-1 Okura, Setagaya-ku, Tokyo 157-8535, Japan. Tel: 81-3-3416-0181; Fax: 81-3-3416-2222.

2 Y. Shimoyama, H. Takeda, S. Yoshihara, M. Kitajima, and S. Hirohashi, unpublished observations.

    ABBREVIATIONS

The abbreviations used are: EC, extracellular subdomain; DMEM, Dulbecco's modified Eagle's medium; PAGE, polyacrylamide gel electrophoresis; PVDF, polyvinylidene difluoride; DiI, 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbocyanine perchlorate.

    REFERENCES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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