This subproject is one of many research subprojects utilizing theresources provided by a Center grant funded by NIH/NCRR. The subproject andinvestigator (PI) may have received primary funding from another NIH source,and thus could be represented in other CRISP entries. The institution listed isfor the Center, which is not necessarily the institution for the investigator.Cell-cell junctions are important in physiological processes, with tight junctions helping to maintain the epithelial cell layer that protects multicellular organisms from the environment. Cell surface adhesion proteins involved in forming these junctions play a role in the loss of attachment, which leads cells to become migratory. We have identified and characterized a novel cell adhesion molecule, Junctional Adhesion Molecule-A (JAM-A), which is expressed at endothelial and epithelial cell tight junctions. Our results implicate JAM-A in the events leading to migratory behavior, including cancer cell metastasis, as well as in subfertility. We therefore propose to test the following hypotheses in this proposal: 1) Metastatic behavior of breast cancer cells is related to the expression level of JAM-A. We will determine the expression of JAM-A in breast cancer cell lines with a range of metastatic potentials. We will compare the expression of JAM-A to the metastatic potential, and use cellular and mouse models to confirm the relationship. 2) Post-translational modifications of JAM-A influence the metastatic ability of breast cancer cells. We will determine if post-translational modification of JAM-A is related to the metastatic behavior of these cells. Again we will utilize in vitro, as well as in vivo, models of tumor metastasis. 3) Signaling through JAM-A regulates the metastatic potential of breast cancer cells. The intracellular signaling pathway induced through JAM-A will be characterized. 4) Reduced expression and/or post-translational modification of JAM-A affect spermiogenesis leading to sperm lacking the protein on the heads and the flagellum. Consequently, there is reduced motility and disruption of the signal transduction and protein phosphorylation properties. We will determine the effect of the absence of JAM-A on basal intracellular calcium in both capacitated and uncapacitated sperm to determine its role in calcium signaling which is involved in both progressive and hyperactivated motility. We will also determine if JAM-A is present in a multi-protein signaling complex with Plasma membrane calcium ATPase4 (PMCA4) and Calcium serine kinase (CASK) which are flagellar signaling molecules. Our results will help define the role of JAM-A in cancer cell metastasis and male subfertility resulting from reduced sperm motility, and can identify therapeutic targets.
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