Oxidative Stress Assay in MM.1S Cells

ATCC MM.1S cells were cultured for 24, 48, and 72 hr with BMS309403 (50 µM), SBFI-26 (50 µM), or combination before staining with 500 nM CellROX for 30 min or 5 µM MitoSOX for 10 min per Thermofisher Scientific protocol. Data acquisition was performed on a Miltenyi MACSquant flow cytometer and data analysis was performed using FlowJo analysis software (BD Life Sciences) with a minimum of 10,000 events collected and gated off forward and side scatter plots.

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Farrell M., Fairfield H., Karam M., D'Amico A., Murphy C.S., Falank C., Pistofidi R.S., Cao A., Marinac C.R., Dragon J.A., McGuinness L., Gartner C.G., Iorio R.D., Jachimowicz E., DeMambro V., Vary C, & Reagan M.R. (2023). Targeting the fatty acid binding proteins disrupts multiple myeloma cell cycle progression and MYC signaling. eLife, 12, e81184.

Publication 2023

MACSquant flow cytometer

Bms309403 Cells Mitosox Sbfi 26

Corresponding Organization :

Other organizations : Maine Medical Center, MaineHealth, Tufts University, University of Maine, Dana-Farber Cancer Institute, Harvard University, University of Vermont, University of New England

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Variable analysis

independent variables

BMS309403 (50 µM)
SBFI-26 (50 µM)
Combination of BMS309403 (50 µM) and SBFI-26 (50 µM)

dependent variables

Oxidative stress levels measured by CellROX (500 nM, 30 min)
Mitochondrial superoxide levels measured by MitoSOX (5 µM, 10 min)

control variables

ATCC MM.1S cells
Staining protocols (CellROX and MitoSOX) as per Thermo Fisher Scientific
Data acquisition on Miltenyi MACSquant flow cytometer
Data analysis using FlowJo software (BD Life Sciences)
Minimum of 10,000 events collected and gated off forward and side scatter plots

controls

No controls explicitly mentioned

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