Skip NavigationSkip to Content
Return Return to Search Results

M-Ras/Shoc2 signaling modulates E-cadherin turnover and cell-cell adhesion during collective cell migration

  1. Author:
    Kota, Pradeep [ORCID]
    Terrell, Elizabeth
    Ritt, Daniel
    Insinna, Christine
    Westlake, Christopher
    Morrison, Deborah [ORCID]

  2. Author Address

    Laboratory of Cell and Developmental Signaling, National Cancer Institute-Frederick, Frederick, MD 21702 pkota@email.unc.edu morrisod@mail.nih.gov., Laboratory of Cell and Developmental Signaling, National Cancer Institute-Frederick, Frederick, MD 21702.,
    1. Year: 2019
    2. Date: Feb 26
    3. Epub Date: 2019 02 11
  2. Journal: Proceedings of the National Academy of Sciences of the United States of America
    1. 116
    2. 9
    3. Pages: 3536-3545
  4. Type of Article: Article
  5. ISSN: 0027-8424
  1. Abstract:

    Collective cell migration is required for normal embryonic development and contributes to various biological processes, including wound healing and cancer cell invasion. The M-Ras GTPase and its effector, the Shoc2 scaffold, are proteins mutated in the developmental RASopathy Noonan syndrome, and, here, we report that activated M-Ras recruits Shoc2 to cell surface junctions where M-Ras/Shoc2 signaling contributes to the dynamic regulation of cell-cell junction turnover required for collective cell migration. MCF10A cells expressing the dominant-inhibitory M-RasS27N variant or those lacking Shoc2 exhibited reduced junction turnover and were unable to migrate effectively as a group. Through further depletion/reconstitution studies, we found that M-Ras/Shoc2 signaling contributes to junction turnover by modulating the E-cadherin/p120-catenin interaction and, in turn, the junctional expression of E-cadherin. The regulatory effect of the M-Ras/Shoc2 complex was mediated at least in part through the phosphoregulation of p120-catenin and required downstream ERK cascade activation. Strikingly, cells rescued with the Noonan-associated, myristoylated-Shoc2 mutant (Myr-Shoc2) displayed a gain-of-function (GOF) phenotype, with the cells exhibiting increased junction turnover and reduced E-cadherin/p120-catenin binding and migrating as a faster but less cohesive group. Consistent with these results, Noonan-associated C-Raf mutants that bypass the need for M-Ras/Shoc2 signaling exhibited a similar GOF phenotype when expressed in Shoc2-depleted MCF10A cells. Finally, expression of the Noonan-associated Myr-Shoc2 or C-Raf mutants, but not their WT counterparts, induced gastrulation defects indicative of aberrant cell migration in zebrafish embryos, further demonstrating the function of the M-Ras/Shoc2/ERK cascade signaling axis in the dynamic control of coordinated cell movement. Copyright © 2019 the Author(s). Published by PNAS.

    See More

  1. Keywords:

External Sources

  1. View Full Text
  2. DOI: 10.1073/pnas.1805919116
  3. PMID: 30808747
  4. View record in Web of Science®
  5. WOS: 000459694400037
  6. PII : 1805919116

Library Notes

  1. Fiscal Year: FY2018-2019
NCI at Frederick

You are leaving a government website.

This external link provides additional information that is consistent with the intended purpose of this site. The government cannot attest to the accuracy of a non-federal site.

Linking to a non-federal site does not constitute an endorsement by this institution or any of its employees of the sponsors or the information and products presented on the site. You will be subject to the destination site's privacy policy when you follow the link.

ContinueCancel