TY - JOUR
T1 - Tumour-associated E-cadherin mutations alter cellular morphology, decrease cellular adhesion and increase cellular motility
AU - Handschuh, Gabriele
AU - Candidus, Sonja
AU - Luber, Birgit
AU - Reich, Ulrike
AU - Schott, Christina
AU - Oswald, Sandra
AU - Becke, Helma
AU - Hutzler, Peter
AU - Birchmeier, Walter
AU - Höfler, Heinz
AU - Becker, Karl Friedrich
N1 - Funding Information:
We are grateful to Drs M Takeichi and N Nagafuchi (Department of Biophysics, Faculty of Science, Kyoto University, Kyoto, Japan) for the transfection plasmid pBATEM. We thank Drs J Behrens, J Huelsken and S Meiners (Max Delbrück Centrum, Berlin, Germany) for technical advice and J Huelsken for the Neuro 2A neuroblastoma cells and the vector pSV2neo. We thank Drs A Luz, M Atkinson (Institut für Pathologie, GSF, Neuherberg, Germany) and G Keller (Institut für Patho-logie, TU-München, Munich, Germany) for helpful discussions, and E Mannweiler (Institut für Pathologie, GSF, Neuherberg, Germany) and E Mentele for excellent technical assistance. The authors are thankful to Dr J Mueller (Institut für Chirurgie, TU-München, München, Germany) for critical reading of the manuscript. This work was supported by a Grant to Dr K-F Becker (Be1501) from the Deutsche Forschungsgemeinschaft (DFG).
PY - 1999/7/29
Y1 - 1999/7/29
N2 - A major function of the cell-to-cell adhesion molecule E-cadherin is the maintenance of cell adhesion and tissue integrity. E-cadherin deficiency in tumours leads to changes in cell morphology and motility, so that E-cadherin is considered to be a suppressor of invasion. In this study we investigated the functional consequences of three tumour-associated gene mutations that affect the extracellular portion of E-cadherin: in-frame deletions of exons 8 or 9 and a point mutation in exon 8, as they were found in human gastric carcinomas. Human MDA-MB-435S breast carcinoma cells and mouse L fibroblasts mere stably transfected with the wild-type and mutant cDNAs, and the resulting changes in localization of E-cadherin, cell morphology, strength of calcium-dependent aggregation as well as cell motility and actin cytoskeleton organization were studied. We found that cells transfected with wild-type E-cadherin showed an epitheloid morphology, while all cell lines expressing mutant E-cadherin exhibited more irregular cell shapes. Cells expressing E-cadherin mutated in exon 8 showed the most scattered appearance, whereas cells with deletion of exon 9 had an intermediate state. Mutant E-cadherins mere localized to the lateral regions of cell-to-cell contact sites. Additionally, both exon 8-mutated E-cadherins showed apical and perinuclear localization, and actin filaments were drastically reduced. MDA-MB-435S cells with initial calcium-dependent cell aggregation exhibited decreased aggregation and, remarkably, increased cell motility, when mutant E-cadherin was expressed. Therefore, we conclude that these E-cadherin mutations may not simply affect cell adhesion but may act in a trans-dominant-active manner, i.e. lead to increased cell motility. Our study suggests that E-cadherin mutations affecting exons 8 or 9 are the cause of multiple morphological and functional disorders and could induce the scattered morphology and the invasive behaviour of diffuse type-gastric carcinomas.
AB - A major function of the cell-to-cell adhesion molecule E-cadherin is the maintenance of cell adhesion and tissue integrity. E-cadherin deficiency in tumours leads to changes in cell morphology and motility, so that E-cadherin is considered to be a suppressor of invasion. In this study we investigated the functional consequences of three tumour-associated gene mutations that affect the extracellular portion of E-cadherin: in-frame deletions of exons 8 or 9 and a point mutation in exon 8, as they were found in human gastric carcinomas. Human MDA-MB-435S breast carcinoma cells and mouse L fibroblasts mere stably transfected with the wild-type and mutant cDNAs, and the resulting changes in localization of E-cadherin, cell morphology, strength of calcium-dependent aggregation as well as cell motility and actin cytoskeleton organization were studied. We found that cells transfected with wild-type E-cadherin showed an epitheloid morphology, while all cell lines expressing mutant E-cadherin exhibited more irregular cell shapes. Cells expressing E-cadherin mutated in exon 8 showed the most scattered appearance, whereas cells with deletion of exon 9 had an intermediate state. Mutant E-cadherins mere localized to the lateral regions of cell-to-cell contact sites. Additionally, both exon 8-mutated E-cadherins showed apical and perinuclear localization, and actin filaments were drastically reduced. MDA-MB-435S cells with initial calcium-dependent cell aggregation exhibited decreased aggregation and, remarkably, increased cell motility, when mutant E-cadherin was expressed. Therefore, we conclude that these E-cadherin mutations may not simply affect cell adhesion but may act in a trans-dominant-active manner, i.e. lead to increased cell motility. Our study suggests that E-cadherin mutations affecting exons 8 or 9 are the cause of multiple morphological and functional disorders and could induce the scattered morphology and the invasive behaviour of diffuse type-gastric carcinomas.
KW - Cell adhesion
KW - E-cadherin
KW - Gastric carcinoma
KW - Morphology
KW - Motility
UR - http://www.scopus.com/inward/record.url?scp=0033615002&partnerID=8YFLogxK
U2 - 10.1038/sj.onc.1202790
DO - 10.1038/sj.onc.1202790
M3 - Article
C2 - 10439038
AN - SCOPUS:0033615002
SN - 0950-9232
VL - 18
SP - 4301
EP - 4312
JO - Oncogene
JF - Oncogene
IS - 30
ER -