Anticancer drug screening: Standardization of in vitro wound healing assay

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Abstract

Introduction: Gliomas are characterized by rapid proliferation and aggressive invasion into normal surrounding brain tissue. In medical laboratories, the in vitro wound healing assay stands out as a simple, easy, inexpensive and affordable method to evaluate cell migration and proliferation. Objective: To standardize the in vitro wound healing assay using antimicrotubule drugs as positive controls. Methods: U87MG glioma cells were seeded at different densities and, after 24 h, the monolayer was scratched using different micropipette tip size to create a gap with no cells. The cells were then treated with colchicine and paclitaxel in culture medium with the presence or absence of fetal bovine serum. The wound was photographed with the aid of an inverted microscope and the wound area was measured using the Image J software. Results: Better defined edges scratches and monolayer with approximately 90% confluence were obtained at 1.5 and 2 × 105cells/well density. The width and area of the scratch were, respectively, 948 μm/2.193221 mm2; 964 μm/2.266 mm2and 1448 μm/3.221 mm2to 10. 200 and 1000 μl micropipette tips. Colchicine inhibited wound closure by 12.6% or 3.4%, both in the presence or absence of serum; paclitaxel 2.4 and 6.7% respectively. Conclusion: Under standardized conditions, colchicine and paclitaxel proved to be efficient positive controls into the in vitro wound healing assay.

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De Almeida, V. M., Bezerra, M. A., Nascimento, J. C., & Amorim, L. M. F. (2019). Anticancer drug screening: Standardization of in vitro wound healing assay. Jornal Brasileiro de Patologia e Medicina Laboratorial, 55(6), 606–619. https://doi.org/10.5935/1676-2444.20190054

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