Citation

  • Authors: Saias, L., Gomes, A., Cazales, M., Ducommun, B., Lobjois, V.
  • Year: 2015
  • Journal: Cancer Res 75 2426-33
  • Applications: in vitro / siRNA / INTERFERin
  • Cell type: HCT 116
    Description: Human colon carcinoma cells
    Known as: HCT116

Method

Cells were cultured in 12-well plates and transfected with 1nM siRNA.Experiments were conducted 3 days after transfection.

Abstract

Cell aggregation is frequently impaired during the growth of primary tumors and the formation of metastatic lesions. Cell aggregation depends on cell-cell adhesion; however, no rigorous approach exists to monitor and quantify it accurately in the absence of the confounding factors of cell-substrate adhesion and the resulting cell motility on the substrate. We report here a highly reproducible, automated, microscopy-based quantification of tumor-cell spheroid formation in the absence of cell-substrate adhesion and use it to characterize cell aggregation dynamics in the early steps of this process. This method is based on fluorescence and bright-field microscopy and on a custom MATLAB program to quantify automatically the cells' aggregation kinetics. We demonstrate that the cell-cell adhesion protein E-cadherin and the desmosome proteins DSG2 and DSC2 are important for aggregation. Furthermore, we show that inhibition or silencing of myosin IIa enhances aggregation, suggesting that cytoskeleton tension inhibits tumor cell aggregation. This work opens new avenues to study the principles that govern multicellular aggregation, to characterize the aggregation properties of various tumor cell types, as well as to screen for drugs that inhibit or promote aggregation.

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