1 Molecular Cell Biology Unit, Department of Molecular Biology, Flanders Interuniversity Institute for Biotechnology (VIB)-Ghent University, B-9000 Ghent, Belgium
2 Department of Pathology, University Hospital Antwerp (UZA), B-2650 Edegem, Belgium
3 Department of Radiotherapy, Nuclear Medicine and Experimental Cancerology, University Hospital Ghent, B-9000 Ghent, Belgium
*Author for correspondence (e-mail: f.vanroy{at}dmb.rug.ac.be)
Accepted May 28, 2001
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SUMMARY |
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Key words: Catenin, Cadherin, Muscle, Heart, Testis
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INTRODUCTION |
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In contrast to the growing family of cadherins (Nollet et al., 2000; Yagi and Takeichi, 2000), the family of -catenins is so far quite small. The
E-catenin protein is ubiquitously expressed, mainly in epithelial tissues.
N-catenin shows about 75% identity to
E-catenin, but its expression is restricted to neural tissues (Hirano et al., 1992). By analogy with
E-catenin, it can also bind to ß-catenin or plakoglobin and is supposed to bind
-actinin and actin. Although vinculin shows much less identity (22%) to
E- or
N-catenin, it shares some properties with
-catenins. Vinculin is mainly found in focal adhesions, where it forms the link between the extracellular matrix-binding integrins and the actin cytoskeleton by binding to both the integrin-binding molecule talin and to F-actin (Burridge and Mangeat, 1984). Vinculin is sometimes found in cell-cell contacts as well, and it may even be able to take over the function of
E-catenin by binding directly to ß-catenin (Hazan et al., 1997). However, vinculin has been reported to bind to a central region of
E-catenin and to be essential for apical junctional organization (Watabe-Uchida et al., 1998). Moreover, vinculin contains a unique central proline-rich hinge domain, which is absent in the
-catenins and which allows the vinculin tail to bind to the head, thus masking some binding sites (Johnson and Craig, 1995). For the recently reported
-catulin (Janssens et al., 1999), the identity to both
-catenins and vinculin is about 25% at the amino acid level, but no functional evidence for adhesive properties of
-catulin has yet been found. In addition to their structural role, it is becoming clear that
-catenins and vinculin also have a regulatory function in the coordination of assembly and disassembly of adherens junctions (Rudiger, 1998).
Here, we report on a novel -catenin with about 55% identity and 70% similarity to other
-catenins. We demonstrate the tissue-specific expression of this
T-catenin and its localization to cell-cell junctions of cardiomyocytes. Moreover, testicular peritubular myoid cells are shown to express
T-catenin. Further, we prove that
T-catenin can functionally restore cell-cell adhesion in colon cancer cells lacking
-catenins. Together, these data indicate that this novel
T-catenin is involved in the formation of specific cell-cell contacts in particular types of muscle cells.
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MATERIALS AND METHODS |
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Cloning of human T-catenin cDNA
A human T-catenin-specific expressed sequence tag (EST) clone was identified by BLAST analysis (Altschul et al., 1990) and requested from the IMAGE consortium UK-HGMP Resource Center (Hinxton, UK). Expression of the corresponding transcript was confirmed by RT-PCR on PC-3 mRNA template using primers MCB967 (5'-TGAGGCAGAAAAAGAAAAGA-3') and MCB968 (5'-AGTGTGGTTAGGCAGGATT-3'). To complete the cDNA sequence we performed two consecutive 5' MarathonTM RACE experiments on a human testis Marathon cDNA preparation (Clontech, Palo Alto, CA). For the first 5' RACE, the gene-specific primer was MCB1027 (5'-AATCTGCCGAGCAAGGACATCCA-3') and the nested primer was MCB1028 (5'-TCAGGCAGTTGAGTCATCTTAGC-3'). RACE-PCR was performed on a Perkin Elmer 2400 thermal cycler (Perkin Elmer, Foster City, CA) following the supplied protocol (touchdown PCR). Obtained RACE fragments were purified from agarose gel using QIAquickTM columns (Qiagen, Chatsworth, CA) and then cloned in the pGEMT® vector (Promega, Madison, WI). The resulting plasmid was called pGEMT-haTctn-RACE1. As the cloned cDNA appeared to be incomplete, a second 5'-RACE experiment was performed with gene-specific primer MCB1254 (5'-ACCCGTGACGATGTGAGCAACTC-3') and nested primer MCB1255 (5'-GAGCTGTCTGCGAAGGTCTCTTG-3'). The obtained fragment was cloned in the pGEMT®-easy vector (Promega), and called pGEMTeasy-haTctn-RACE2.
All DNA sequences were determined by the dideoxy chain termination method (Sanger et al., 1977), using fluorescent dye terminators in a 377ABI automated DNA sequencer (Applied Biosystems, Foster City, CA). Sequences were assembled and compared by use of the software packages DNAstar (DNASTAR, Madison, WI) and Staden gap4 (Bonfield et al., 1995). Protein alignments and amino acid similarities were calculated using the CLUSTAL W program (Higgins and Sharp, 1989; Thompson et al., 1994) and GCG software. Alignments were shaded using the WWW-BOXSHADE server (http://ulrec3.unil.ch/softward/BOX_form.html).
Expression analysis by RT-PCR
Expression analysis using the human Rapid-Scan panel (OriGene Technologies, Rockville, MD) was performed on 100-times diluted template, followed by nested PCR (1/10 of the end volume of the first reaction was used). Primers MCB967 (5'-TGAGGCAGAAAAAGAAAAGA-3') and MCB968 (5'-AGTGTGGTTAGGCAGGATT-3') were used for the first PCR, yielding a product of 743 bp. For nested PCR, primers MCB967 (5'-TGAGGCAGAAAAAGAAAAGA-3') and MCB1010 (5'-GCTGAGCCTCGTCTGAC-3') were combined, yielding a smaller product of 630 bp. The end-point determination method used does not allow a reliable determination of expression levels to be deduced from the amount of PCR product visualized on gel. Therefore, visual presence of a signal (even weak) was scored as positive, and complete absence was scored as negative. As a control, an E-catenin-specific product of 747 bp was amplified with primers MCB53 (5'-CTTCGGGCCTCTGGAATTTA-3') and MCB73 (5'-CGACATCAGGGTGCTGTAGG-3'). Amplified products were checked for specificity by sequence analysis, showing that the double bands observed for heart and testis after nested RT-PCR indeed correspond to the larger primary product and the smaller nested product predicted.
For RT-PCR analysis of mouse tissues, RNA was prepared from different tissues with the RNAeasy method (Qiagen) and cDNA was prepared using a commercial kit (Life Technologies, Paisley, UK). For mouse T-catenin, primers MCB2461 (5'-CCCCAATGTTTT-ATGTTAT-3') and MCB2463 (5'-GGGGAGAACTCATCGTAT-3') were designed on the sequence of an EST clone (GenBank accession no. AW556211), resulting in amplification of a 442-bp product. For mouse
E-catenin (GenBank accession no. NM_009818), a 733-bp product was amplified with primers MCB2636 (5'-GAAGGCCCCTGAGAAGAA-3') and MCB2637 (5'-CCCGAATAAAGCAACTCCAT-3'). For mouse
N-catenin (GenBank accession no. NM_009819) an 858-bp product was amplified with primers MCB2479 (5'-GCCCTGATTGAGTTTGATAA-3') and MCB2480 (5'-CCCAGCTTCATAGTTCTCC-3'). As a control, a 452-bp fragment of mouse GAPDH was amplified with primers MCB2219 (5'-ACCACAGTCCATGCCATCAC-3') and MCB2220 (5'-TCCACCACCCTGTTGCTGTA-3').
Eukaryotic expression plasmids
After completion of plasmid constructs as described below, all clones were checked by DNA sequencing. For all PCRs, Pfu polymerase (Stratagene, La Jolla, CA) with proofreading activity was used. A PCR product of 1134 bp was synthesized with primers MCB1607 (5'-AGAATTCTCAGCTGAAACACCAATCAC-3') and MCB1609 (5'-AGGATCCTGCGAAGGTCTCTTGTCT-3') using the pGEMTeasy-haTctn-RACE2 clone as a template. This product, restricted with EcoRI and PstI, was combined with a PstI-SspI fragment of pGEMT-haTctn-RACE2, an SspI-BglII fragment from pGEMTeasy-haTctn-RACE1, and a BglII-SalI fragment of a 3' overlapping PCR product generated with primers MCB1610 (5'-GGATGATAATCAATTTGTGGACATCTC-3') and MCB1608 (5'-GGGATCCGTAGATTTGTCTTCCTCTAA-3') on RNA from the PC-3 prostate cancer cell line. The full-length human T-catenin cDNA was inserted in the EcoRI-SalI-digested pEGFPC2 vector (Clontech), in order to obtain an in-frame N-terminal fusion with the GFP protein. The resulting plasmid was called pEGFPC2-haTctn(179-2860). An EcoRI-BstEII fragment from clone pGEMT-RACE2 was combined with a BstEII-NotI fragment of pEGFPC2-haTctnCTN(179-2860) in the EcoRI-NotI-digested vector pEF6MycHisA (Invitrogen, San Diego, CA), yielding construct pEF6MH-haTctn(1-2860) encoding a C-terminal fusion between human
T-catenin and the Myc and His epitopes.
Screening of a human fetal kidney 5' stretch cDNA library in vector DR2 (Clontech) with an
E-catenin-specific probe resulted in the isolation of the pDR2
ECTN plasmid, from which an Eco47III-SalI fragment corresponded to the full-length
E-catenin cDNA (GenBank accession no. D14705). The latter fragment was purified and ligated in the EcoRI-SalI-digested pEGFPC2 vector (Clontech), yielding plasmid pEGFPC2-haEctn(69-3454).
A full-length cDNA fragment of human N-catenin (GenBank accession No. M94151) was prepared from plasmid pPN-hANCTN (Claverie et al., 1993), kindly provided by C. Petit (Institut Pasteur, Paris). This fragment was then cloned in the EcoRI-SalI-digested pEGFPC2 vector (Clontech), yielding plasmid pEGFPC2-haNctn(39-2885).
Transfection experiments
For vaccinia virus-mediated transient overexpression, -catenins were cloned in the pE/L-GFP vector (Frischknecht et al., 1999). Cells were transfected with Lipofectin (Life Technologies) and simultaneously co-infected with vaccinia virus strain
A36R, which does not make actin tails (Parkinson and Smith, 1994). At 4 to 30 hours after transfection, high levels of expression under control of the vaccinia virus early/late promoter (E/L) (Chakrabarti et al., 1997) were obtained of the cloned cDNA, N-terminally fused to GFP. To this end, human
T-catenin cDNA was amplified with Taq+Precision polymerase (Stratagene) using primers containing a 5' NotI site and a 3' EcoRI site (MCB2386, 5'-GGGGGCGGCCGCGGAGGGTCAGCTGAAACACCAATCACATTG-3' and MCB2387, 5'-CCCCGAATTCGCCGTGTGGTTAGGCAGGATTTTGTCATATAG-3') and cloned into the NotI-EcoRI sites of the pE/L-GFP vector, yielding plasmid pE/L-GFP-haTctn(179-2913).
HEK-293 cells were transiently transfected by the calcium phosphate method. For stable transfection of HCT-8/R1 carcinoma cells, 4x106 cells were electroporated (Easyject; Eurogentec, Seraing, Belgium) with 10 µg of plasmid pEF6MH-haTctn(1-2860). Cells were plated and cultured in the presence of 6 µg/ml blasticidin (Invitrogen) to select for stable transfectants. Colonies of blasticidin-resistant cells were isolated and tested by immunofluorescence and western blotting for expression of T-catenin. One positive clone was isolated and called HCT-8/R1/T31. As a negative control we transfected HCT-8/R1 cells with the empty pEF6MH vector, resulting in stable clones called HCT-8/R1/1743. As reported previously (van Hengel et al., 1997), related HCT-8/E11R1 cells were stably transfected with
N-catenin cDNA and a positive clone was designated HRpC
N2.
Antibodies
For the generation of polyclonal antibodies, peptide #952 with sequence C-KIHPLQVMSEFRGRQIY, corresponding to the C-terminus of the human T-catenin protein, was coupled to keyhole-limpet hemocyanin (Sigma, St Louis, MO) and injected into each of three rabbits using Titermax (Sigma) as adjuvant. Boosts were given with intervals of minimum two weeks. Sera were tested by ELISA on the peptide used for injection, using nonrelevant peptide as a negative control. For western blotting, a dilution of 1:1000 was used and recognition of
T-catenin was inhibited by incubation of the polyclonal antibody in blocking solution containing 0.5 to 2.5% antigenic peptide for 1 hour prior to use.
Monoclonal antibodies were generated by coupling N-terminal peptide #892, with sequence C-VANKSDLQKTYQKL, to keyhole-limpet hemocyanin, followed by injection into C57Bl/6 mice. Boosts were given with intervals of 2 weeks, and sera were tested by peptide-ELISA until a titer of 1:10,000 without loss of reactivity was obtained after 6 weeks. Hybridomas were generated by fusion of spleen cells with Sp20_Ag14 myeloma cells. Supernatants of hybridoma cell lines, positive in peptide-ELISA, were tested by western blotting and immunofluorescence for recognition of the T-catenin protein, fused at its N-terminus to GFP, in lysates of various cells transfected with plasmid pEGFPC2-haTctn(179-2860). One hybridoma cell line, designated 892_24D2S after subcloning, was deposited with the Belgian Coordinated Collections of Microorganisms (BCCMTM) (no. LMBP 5537CB) and used for further analysis.
Other primary antibodies used were polyclonal E-catenin- and ß-catenin-specific antibodies (Sigma), monoclonal
E-catenin- and ß-catenin-specific antibodies (Transduction, Lexington, KY), anti-E-cadherin monoclonal antibodies HECD-1 (Takara Biochemicals, Otsu, Japan) and MB2 (Bracke et al., 1993), anti-N-cadherin monoclonal antibody (Zymed, San Francisco, CA), monoclonal anti-desmin antibody clone 33 (Biogenex, San Ramon, CA), anti-desmoglein clone 10G11 (Progen, Heidelberg, Germany), anti-ZO-1 (Zymed) and anti-Myc-tag clone 9E10 (Oncogene, Cambridge, MA).
SDS-PAGE and western blot analysis
Protein lysates from various mouse tissues were prepared by isolating the tissues from normal BALB/c mice and mixing them in Laemmli buffer (Laemmli, 1970). Debris was removed by centrifugation and protein concentration was measured by the BioRad DC kit (BioRad, Richmond, CA). Lysates from subconfluent cultures of cell lines were also prepared in Laemmli buffer, followed by sonication and centrifugation. Of each protein lysate, 40 µg was diluted with 6x sample buffer (0.35 M Tris-HCl, pH 6.8, 10.28% SDS, 36% glycerol, 5% ß-mercaptoethanol, 0.012% bromophenol blue), boiled for 5 minutes and subjected to separation on 10% polyacrylamide gels. Proteins were transferred onto Immobilon-P membranes (Millipore, Bredford, MA) and blocked with 5% nonfat dry milk, 0.1% Tween-20 in Tris-buffered saline buffer (100 mM Tris-HCl, pH 7.4, 1.4 M NaCl) prior to incubation with the primary antibody. Detection was carried out by phosphatase-coupled secondary antibodies (Sigma) and nitroblue tetrazolium/5-bromo-4-chloro-3-indolyl phosphate (NBT/BCIP) as a substrate.
For co-immunoprecipitation, lysates of transfected HEK-293 cells were prepared in PBS containing 1% Nonidet P-40 and a protease inhibitor cocktail (Boehringer). Lysates of mouse tissues were prepared in extraction buffer containing 25 mM Tris/HCl (pH 7.5), 1 mM EDTA, 1 mM EGTA, 100 mM NaCl, 1% Triton X-100, 0.5% Nonidet P-40 and the protease inhibitor cocktail. Lysate (800 µg) was incubated overnight with 4 µg of the respective antibody, after which 100 µl of 50% protein-G Sepharose (Amersham Pharmacia Biotech, Rainham, UK) was added to monoclonal antibodies, whereas protein-A Sepharose (Amersham Pharmacia Biotech) was added to polyclonal antibodies. After 2 hours of incubation, the Sepharose beads were washed three times with PBS containing 0.1% Nonidet P-40, followed by boiling for 5 minutes in Laemmli buffer. Samples were split in two parts before being subjected to SDS-PAGE and western blotting. On these western blots, protein was detected by the ECL detection system using secondary antibodies coupled to horseradish peroxidase (Amersham Pharmacia Biotech).
Immunodetection in cryosections of human tissues
For immunohistochemistry, frozen sections of human heart and testis tissues were air dried and fixed in aceton at 4°C for 10 minutes. The sections were washed in PBS and preincubated with 10% goat serum for 10 minutes. They were then incubated for 30 minutes with crude monoclonal 892_24D2S hybridoma supernatant, which was diluted in PBS with 1% BSA, or with clone 33 anti-desmin antibodies. The secondary antibody used was biotin-labeled goat-anti-mouse Ig (Dako, Carpinteria, CA), which was subsequently linked to streptavidin-biotin complex coupled to horseradish peroxidase. Detection was carried out by a 5-minute incubation with the chromogenic peroxidase substrate diaminobenzidine (Biogenex). Cell nuclei were counterstained with hematoxylin, after which the slides were dehydrated in alcohol, cleared in toluol and mounted.
For double immunofluorescent staining, frozen sections were air dried, fixed in acetone at 4°C for 10 minutes, washed in PBS and preincubated with 10% goat serum for 10 minutes. The slides were then incubated for 45 minutes with mixtures of primary antibodies diluted in PBS: either 1:5 monoclonal antibody 892_24D2S plus 1:500 polyclonal anti-E-catenin, or 1:500 polyclonal antibody #952 plus 1:500 monoclonal anti-N-cadherin. The secondary goat anti-mouse IgG and goat anti-rabbit IgG antibodies used were labeled with FITC or TRITC (Santa Cruz Biotechnology, Santa Cruz, CA), or with Alexa 488 or Alexa 594 (Molecular Probes, Eugene, OR).
Immunocytochemistry of cell cultures
Cells were grown on glass coverslips until confluency, rinsed briefly with PBS and fixed with either ice-cold methanol for 1 minute, or with 3% paraformaldehyde (Merck, Darmstadt, Germany) for 10 minutes at room temperature, followed by permeabilization in 0.2% Triton X-100 (Sigma) for 2 minutes. Cells were then incubated for 30 minutes with primary antibody diluted in blocking solution (20 mM Tris/HCl pH 7.5, 154 mM NaCl, 2 mM EDTA, 2 mM MgCl2, with 1% BSA and 1% goat serum), washed in PBS, and incubated for 30 minutes with secondary antibodies diluted in blocking solution. Secondary anti-mouse IgG or anti-rabbit IgG antibodies were coupled to either Alexa 594 or Alexa 488 (Molecular Probes). Finally, cells were treated for 10 seconds with a 4'-6-diamidine-2-phenylindole-dihydrochloride solution (DAPI; Roche Diagnostics, Mannheim, Germany) to mark nuclear DNA, followed by mounting in Vectashield (Vector Laboratories, Burlingame, CA) to prevent photobleaching. Samples were examined with a Zeiss Axiophot microscope and images were recorded with a high-performance charge-coupled digital camera (Cohu, San Diego, CA) and NIH image software (version 1.62), or with a MicroMAX camera (Princeton, Trenton, NJ) and MetaMorph software (Image Universal Corporation, New York, NY).
Aggregation assays
Cell-cell adhesion was numerically evaluated in a fast aggregation assay as described before (Bracke et al., 1993). In brief, cultures were dissociated into single-cell suspensions under E-cadherin-saving conditions using collagenase. They were incubated under Gyrotory shaking (New Brunswick Scientific, New Brunswick, NJ) at 80 rpm for 30 minutes in an isotonic buffer containing either 1 mM EGTA or 1.25 mM Ca2+. E-cadherin could be functionally blocked by treatment with MB2 anti-cadherin monoclonal antibody, starting 30 minutes before aggregation at 4°C and continued throughout aggregation at 37°C. The volume distribution (expressed as % of the total cell volume) in function of the particle diameter was measured by an LS200 particle size analyzer (Coulter Electronics Ltd, Luton, UK), at the start of the incubation at 37°C (t0) and after 30 minutes (t30). The Kolmogoronov-Smirnov test was applied to cumulative fast aggregation curves to analyze statistical differences.
Slow aggregation was performed as described (Boterberg et al., 2000). Briefly, single-cell suspensions were seeded onto a semi-solid agar medium. After 24 hours, aggregate formation was evaluated subjectively by phase-contrast microscopy.
For the compaction and decompaction assays, cells were seeded at a density of 6x105 cells/6 ml of RPMI supplemented with 10% fetal bovine serum. The suspended cells were incubated on a Gyrotory shaker (New Brunswick, NJ) at 80 rpm for 3 days. Aggregate formation was evaluated, after which the multicellular spheroids were dissociated by passing 30 times through Pasteur pipettes with a diameter of 1.5 mm (Takeda et al., 1995). Compaction and decompaction were evaluated qualitatively by phase-contrast microscopy and quantitatively by measuring the volume distribution (% of total cell volume) in function of the particle diameter using an LS200 particle size analyzer (Coulter).
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RESULTS |
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We then investigated the localization of T-catenin protein in frozen tissue sections of human heart and testis. In human cardiomyocytes,
T-catenin protein was clearly located at cell-cell contacts (i.e. intercalated discs; Fig. 3). In double labelling experiments, it co-localized with
E-catenin (Fig. 3A) as well as N-cadherin (Fig. 3B). The muscle marker desmin could be detected at both intercalated discs and sarcomeric Z-lines, whereas
T-catenin expression was confined to intercalated discs (Fig. 3C). In human testis,
T-catenin protein was detected mainly in spindle-shaped cells surrounding testicular tubuli (Fig. 4). Interestingly,
T-catenin did not co-localize here with
E-catenin, as the latter showed an abundant intratubular expression pattern (Fig. 4A). The
T-catenin-expressing cells in testis correspond to desmin-positive cells (Fig. 4B), and therefore could be identified as peritubular myoid cells. These stainings suggest that
T-catenin expression is confined to specific muscle cell types, although detailed immunohistological studies of additional tissues are warranted in this respect.
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DISCUSSION |
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The 3D structure of an N-terminal fragment of the E-catenin protein was resolved recently and shown to consist of antiparallel
-helices, which together form a four-helix bundle either by homodimerization or by binding to ß-catenin (Pokutta and Weis, 2000). A typical feature of this
E-catenin structure is a tandem kink of 30°, generated by two proline residues in helices
3 and
4, respectively (marked by [P] in Fig. 1A). It is noteworthy that such proline residues are completely absent from the
N-catenin protein sequence, while only one is present in the
T-catenin sequence. The domain for binding to ß-catenin is located in the very N-terminal part of
-catenins. Although it was reported that a small fragment, corresponding to
-helix-2a (Fig. 1A), can bind to ß-catenin (Huber et al., 1997), it was more recently proposed on the basis of the 3D structure of the
E-catenin fragment, that
-helix-0 is also needed for binding to ß-catenin (Pokutta and Weis, 2000). The amino acid sequences of both
-helix-0 and
-helix-2a seem to be well conserved across the three
-catenin types, along with their ability to bind to ß-catenin.
As shown by RT-PCR and immunoblotting analysis, T-catenin shows a restricted tissue-specific expression pattern, with remarkably abundant mRNA levels in heart and testis. Protein levels were particularly high in heart. In addition, specific transcripts were detected in brain and skeletal muscle of both man and mouse, and in tongue, uterus and ovary of mouse; this was confirmed at the protein level. Some discrepancy was observed between mRNA expression levels in kidney and liver of man versus mouse. This could be due partly to species differences. A wide variety of cell lines was checked by RT-PCR and western blotting, but all lacked detectable
T-catenin (data not shown). Overall, our expression analysis showed clearly that
T-catenin is more tissue-specific than
E-catenin or ß-catenin, although less tissue-restricted than
N-catenin. The expression of
T-catenin in heart is particularly striking. In this context, it is remarkable that metavinculin, a member of the
-catenin/vinculin family, is specifically expressed in cardiac and smooth muscle (Belkin et al., 1988; Gimona et al., 1987).
The polyclonal and monoclonal antibodies generated by us against T-catenin peptides turned out to be specific without crossreaction with
E-catenin or
N-catenin. Likewise, all
-catenin-specific antibodies tested hardly crossreacted with
T-catenin protein in western blot analyses. This means that in all previously reported analyses of adhesion complexes, including the specialized intercalated discs between individual heart muscle cells,
T-catenin protein was probably not detected. The availability of
T-catenin-specific antibodies without crossreactivity will allow previous findings to be re-evaluated. In intercalated discs N-cadherin is the most important junction molecule (Volk and Geiger, 1984; Volk and Geiger, 1986). N-cadherin is known to be linked at its cytoplasmic site to ß-catenin or plakoglobin (Hertig et al., 1996), but much less is known about the particular link between this complex and the actin cytoskeleton, more particularly the heart-specific myofibrils. It has been suggested that this link is very important, as plakoglobin null-mutant embryos die from embryonic day 10.5 onwards, owing to an impairment in the architecture of myocardiac intercalated discs (Bierkamp et al., 1996; Ruiz et al., 1996). We detected colocalization of
E- and
T-catenins in intercalated discs.
In human testis cryosections, we detected T-catenin protein in peritubular myoid cells. Interestingly,
E-catenin is not co-localizing here with
T-catenin as it is present in intratubular cells. This differential localization points towards a specific function for
T-catenin. It was shown for peritubular myoid cells in the mouse that they express P-cadherin and ß-catenin at their cell membranes from day 15 after birth (Lin and DePhilip, 1996), when actin filaments are fully organized in a characteristic orthogonal pattern (Vogl et al., 1995). In maturating peritubular cells of the rat,
E- and ß-catenin were detected but not plakoglobin (Byers et al., 1994). We may propose a role for
T-catenin in the formation of a complex between P-cadherin and F-actin, thus stabilizing the cell-cell contacts between testicular peritubular myoid cells.
To show functionality of T-catenin in cell-cell adhesion complexes, expression of ectopic
T-catenin in HCT-8/R1 cells lacking
-catenins was found to functionally restore adhesive properties. Vaccinia virus-mediated transient overexpression of
T-catenin in these cells clearly resulted in recruitment of ß-catenin to cell-cell contact sites. Stable transfection with a plasmid encoding Myc-tagged
T-catenin resulted in restoration of the cadherin-based adhesion complex, but also of structures resembling tight junctions and desmosomes. We showed restoration of strong cell-cell adhesiveness in both fast and slow aggregation assays. Thus, we showed that
T-catenin, like
E- and
N-catenin, functions in cadherin-mediated cell-cell adhesion by providing the necessary link between ß-catenin and the actin cytoskeleton.
The fact that T-catenin co-immunoprecipitated with ß-catenin from testis and heart tissues points towards a specific function in adhesion complexes of these tissues. The relevance of co-expression of
T- and
E-catenin in cardiomyocytes remains to be elucidated. It is conceivable that stronger anchoring of adhesion complexes to the actin cytoskeleton is needed in heart muscle tissues, where
T-catenin is mainly expressed.
T-catenin may reinforce the cell-cell adhesion junctions by forming molecular complexes similar to but tighter than those containing
E-catenin. Furthermore, it is possible that
T-catenin distinguishes itself from other
-catenins by binding to specific interaction partners.
In summary, we report an interesting novel member of the -catenin family. Although
T-catenin can be detected in the same tissues as
E-catenin, enriched levels, especially in cardiomyocytes and testicular peritubular myoid cells, point at a crucial role in tissue-specific cell-cell adhesion junctions. Introduction of ectopic
T-catenin in carcinoma cells with defective
E-catenin expression restores functional cadherin-catenin complexes. Further analysis of
T-catenin may contribute to understanding how particular tissues achieve different ways of cell-cell adhesion by use of specific
-catenins. It will be challenging to discover
T-catenin-specific binding partners and functions that are not shared by the other
-catenins.
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ACKNOWLEDGMENTS |
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