Functional Cis-Heterodimers of N- and R-Cadherins

Author:

Shan Wei-Song1,Tanaka Hidekazu1,Phillips Greg R.1,Arndt Kirsten1,Yoshida Mika1,Colman David R.1,Shapiro Lawrence2

Affiliation:

1. Department of Biochemistry and Molecular Biology, Programs in Cell Adhesion and Structural Biology

2. Department of Physiology and Biophysics, The Mount Sinai School of Medicine of New York University, New York, New York 10029

Abstract

Classical cadherins form parallel cis-dimers that emanate from a single cell surface. It is thought that the cis-dimeric form is active in cell–cell adhesion, whereas cadherin monomers are likely to be inactive. Currently, cis-dimers have been shown to exist only between cadherins of the same type. Here, we show the specific formation of cis-heterodimers between N- and R-cadherins. E-cadherin cannot participate in these complexes. Cells coexpressing N- and R-cadherins show homophilic adhesion in which these proteins coassociate at cell–cell interfaces. We performed site- directed mutagenesis studies, the results of which support the strand dimer model for cis-dimerization. Furthermore, we show that when N- and R-cadherins are coexpressed in neurons in vitro, the two cadherins colocalize at certain neural synapses, implying biological relevance for these complexes. The present study provides a novel paradigm for cadherin interaction whereby selective cis-heterodimer formation may generate new functional units to mediate cell–cell adhesion.

Publisher

Rockefeller University Press

Subject

Cell Biology

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