AutoDock scoring function provided a preliminary ranking for the compounds. The study of cell migration is essential for understanding a variety of processes including wound repair, immune response and tissue homeostasis; importantly, aberrant cell migration can result in various pathologies. However, the relationship between cytoskeletal dynamics, including actin network growth, contractility, and adhesion, to cell shape and migration remains incompletely understood. Abl family tyrosine kinases are ubiquitous non-receptor tyrosine kinases involved in signal transduction. They can interact with other VE-821 cellular components through multiple functional domains for filamentous and globular actin binding, as well as through binding phosphorylated tyrosines, polyproline rich regions, DNA, and microtubules ). Abl family tyrosine kinases have also been found to regulate cell migration. In some cases, Abl family kinases have been reported to promote actin polymerization and migration as well as filopodia formation during cell spreading. By contrast, in other studies Abl was found to restrain lamellipodia extension or inhibit initial cell attachment to the substrate. Abl family kinases have been suggested to regulate cell adhesion size and stress fiber formation ; Li and Pendergast recently reported that the Abl family member Arg, could disrupt CrkII-C3G complex formation to reduce b1-integrin related adhesion formation. Thus, a complete understanding of how Abl family kinases regulate cell migration is lacking. In this study, we report that Gleevec, an Abl family kinase inhibitor that is used as a chemotherapeutic agent for leukemia, produces a profound change in the shape and migration of the rat Nara bladder tumor cells plated on collagen-coated substrates. Within 20 min of PCI-32765 Gleevec treatment the majority of NBT-II cells develop a new D-shaped morphology and start migrating more rapidly and with greater persistence. The new morphology is characterized by stronger cellsubstrate adhesion and an increase in the size and number of discrete adhesions which at the leading margin turnover more rapidly. RhoA activity in Gleevec-treated cells was increased which, via myosin activation, led to an increase in the magnitude of total traction forces applied to the substrate. Upon Gleevec treatment, these chemical and physical alterations combined to produce the dramatic change in morphology and migration. Here, we show that inhibition of Abl family kinase activity with Gleevec produced a rapid and remarkable change in cell morphology and migration in which cells spread out a thin, extended lamella and migrated faster and with more persistence with some similarities to fish and amphibian keratocyte migration. In addition, this rapidly spreading, very thin lamella is similar to the rapid and extensive, “pancake” spreading of fibroblasts derived from Abl null mice. Associated with the Gleevec phenotype was an increase in RhoA activity, increased global cell adhesion strength, a pronounced change in adhesion patterns and an increase in total traction applied to the substrate. This transient re-localization also occurs in NIH3T3 cells, where a fraction of the cellular Abl associates with the focal adhesion proteins, paxillin and Grb2. Abl family kinases have also been reported to reduce initial cell attachment to the substrate.