Non-cysteine linked MUC1 cytoplasmic dimers are required for Src recruitment and ICAM-1 binding induced cell invasion

Ashlyn J Bernier; Jing Zhang; Erik Lillehoj; Andrew R E Shaw; Nirosha Gunasekara; Judith C Hugh

doi:10.1186/1476-4598-10-93

Non-cysteine linked MUC1 cytoplasmic dimers are required for Src recruitment and ICAM-1 binding induced cell invasion

Mol Cancer. 2011 Jul 28:10:93. doi: 10.1186/1476-4598-10-93.

Authors

Ashlyn J Bernier¹, Jing Zhang, Erik Lillehoj, Andrew R E Shaw, Nirosha Gunasekara, Judith C Hugh

Affiliation

¹ Department of Laboratory Medicine and Pathology, 3-70 Heritage Medical Research Centre, University of Alberta, Edmonton, AB, T6G 2S2, Canada.

Abstract

Background: The mucin MUC1, a type I transmembrane glycoprotein, is overexpressed in breast cancer and has been correlated with increased metastasis. We were the first to report binding between MUC1 and Intercellular adhesion molecule-1 (ICAM-1), which is expressed on stromal and endothelial cells throughout the migratory tract of a metastasizing breast cancer cell. Subsequently, we found that MUC1/ICAM-1 binding results in pro-migratory calcium oscillations, cytoskeletal reorganization, and simulated transendothelial migration. These events were found to involve Src kinase, a non-receptor tyrosine kinase also implicated in breast cancer initiation and progression. Here, we further investigated the mechanism of MUC1/ICAM-1 signalling, focusing on the role of MUC1 dimerization in Src recruitment and pro-metastatic signalling.

Methods: To assay MUC1 dimerization, we used a chemical crosslinker which allowed for the detection of dimers on SDS-PAGE. We then generated MUC1 constructs containing an engineered domain which allowed for manipulation of dimerization status through the addition of ligands to the engineered domain. Following manipulation of dimerization, we immunoprecipitated MUC1 to investigate recruitment of Src, or assayed for our previously observed ICAM-1 binding induced events. To investigate the nature of MUC1 dimers, we used both non-reducing SDS-PAGE and generated a mutant construct lacking cysteine residues.

Results: We first demonstrate that the previously observed MUC1/ICAM-1 signalling events are dependent on the activity of Src kinase. We then report that MUC1 forms constitutive cytoplasmic domain dimers which are necessary for Src recruitment, ICAM-1 induced calcium oscillations and simulated transendothelial migration. The dimers are not covalently linked constitutively or following ICAM-1 binding. In contrast to previously published reports, we found that membrane proximal cysteine residues were not involved in dimerization or ICAM-1 induced signalling.

Conclusions: Our data implicates non-cysteine linked MUC1 dimerization in cell signalling pathways required for cancer cell migration.

Publication types

Research Support, Non-U.S. Gov't
Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

Breast Neoplasms / genetics
Breast Neoplasms / metabolism
Breast Neoplasms / pathology*
Carcinoma / genetics
Carcinoma / metabolism
Carcinoma / pathology*
Cell Line, Tumor
Cysteine / genetics
Cysteine / metabolism
Female
HEK293 Cells
Humans
Intercellular Adhesion Molecule-1 / metabolism*
Models, Biological
Mucin-1 / chemistry
Mucin-1 / genetics
Mucin-1 / metabolism
Mucin-1 / physiology*
Neoplasm Invasiveness
Protein Binding / drug effects
Protein Binding / genetics
Protein Multimerization / physiology*
RNA, Small Interfering / pharmacology
src-Family Kinases / genetics
src-Family Kinases / metabolism*

Substances

Mucin-1
RNA, Small Interfering
Intercellular Adhesion Molecule-1
src-Family Kinases
Cysteine