AI Article Synopsis

  • Loss of KAI1, a tumor-suppressor protein, is linked to worse outcomes in cancer patients, especially as its presence diminishes in metastases.
  • KAI1 interacts with integrin αvβ3 to inhibit ovarian cancer cell behavior, while a variant called KAI1-splice exhibits the opposite effect by promoting cell migration and proliferation.
  • The KAI1-splice variant not only diminishes KAI1's tumor-suppressive capabilities but also enhances functions that favor tumor growth and spread due to increased signaling through the epidermal growth factor receptor.

Article Abstract

Loss or downregulation of the tumor-suppressor KAI1 correlates with poor cancer patient prognosis. KAI1 functions by interacting with other proteins, including integrin cell adhesion and signaling receptors. We previously showed that KAI1 physically and functionally crosstalks with the tumor-biologically relevant integrin αvβ3, thereby suppressing ovarian cancer cell migration and proliferation. Interestingly, in metastases, a KAI1 splice variant had been identified, indicating poor patient prognosis. Thus, we here characterized differential effects of the two KAI1 proteins upon their cellular restoration. Opposite to KAI1, KAI1-splice reduced αvβ3-mediated cell adhesion, thereby inducing cell migration. This was accompanied by elevated αvβ3 levels and drastically elevated focal adhesion kinase activation, however, without any obvious colocalization with αvβ3, as observed for KAI1. Moreover, codistribution of KAI1 with the cell/cell-adhesion molecule E-cadherin was abrogated in KAI1-splice. Whereas KAI1 diminished cell proliferative activity, KAI1-splice prominently enhanced cell proliferation concomitant with elevated transcription and cell-surface expression of the epidermal growth factor receptor. Thus KAI1-splice does not only counteract the tumor-suppressive actions of KAI1, but - beyond that - promotes αvβ3-mediated biological functions in favor of tumor progression and metastasis.

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Source
http://dx.doi.org/10.1016/j.cellsig.2014.11.028DOI Listing

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