Characterization of Cx26-Expressing HeLa Cells

Membranes were developed with alkaline phosphatase-conjugated secondary antibodies, and signals were visualized using either the Alpha Innotech FluorChem HD2 Imaging System (San Leandro, CA, USA) or the FluoroChem M system (Cell Biosciences, Preston, Australia). The following antibodies were purchased from Santa Cruz Biotechnology (Dallas, TX, USA): Cx26 (sc-130729), Il1β (sc-52012), P-AKT (sc-7985R), AKT (sc-5298), GSK3β (sc-81462), and β-actin (sc-47778). GAPDH (#14C10) was from Cell Signaling Technology (Danvers, MA, USA). Primary antibodies were used at a 1:1000 dilution with Santa Cruz HRP-conjugated anti- mouse and anti-rabbit secondary antibodies at 1:3000. We tested both the change in protein expression by western blot and the change in the extent of coupling by the dye preloading assay which is a functional assay for dye transfer between cells. We utilized parental HeLa cells that do not express gap junctions and HeLa cells that are stably transfected with Cx26 [31 (link)]. We have characterized HeLa26 cells according to growth and migration properties [32 (link), 50 (link)].

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Bagati A., Hutcherson T.C., Koch Z., Pechette J., Dianat H., Higley C., Chiu L., Song Y., Shah J., Chazen E., Nicolais A., Casey P., Thompson K., Burke K., Nikiforov M.A., Zirnheld J, & Zucker S.N. (2020). Novel combination therapy for melanoma induces apoptosis via a gap junction positive feedback mechanism. Oncotarget, 11(37), 3443-3458.

Publication 2020

FluorChem HD2 Imaging System Il1β P-AKT GSK3β β-actin GAPDH HRP-conjugated anti- mouse and anti-rabbit secondary antibodies

Actin Alkaline phosphatase Anti antibodies Antibodies Assay Cells Cx26 Dilution Gap junctions Gapdh Gsk3β Hela cells Il1β Membranes Mouse Parental Protein change Rabbit Sc 52012 Western blot

Corresponding Organization :

Other organizations : Roswell Park Comprehensive Cancer Center, D'Youville College, University at Buffalo, State University of New York

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Variable analysis

independent variables

Expression of Cx26 protein in HeLa cells

dependent variables

Protein expression levels of Cx26, Il1β, P-AKT, AKT, GSK3β, and β-actin measured by Western blot
Extent of coupling measured by dye preloading assay

control variables

Parental HeLa cells that do not express gap junctions
HeLa cells stably transfected with Cx26
Primary antibody dilution at 1:1000
Secondary antibody dilution at 1:3000

controls

Positive control: HeLa cells stably transfected with Cx26
Negative control: Parental HeLa cells that do not express gap junctions

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