I would like to measure the levels of specific cell surface proteins following treatment with an antibody drug. However, the drug itself occupies the same epitope (or a close enough epitope) to inhibit staining with fluorescently labeled antibodies to the same target protein. I'd like to know if there is a way to wash the antibody/drug from my treated cells so that they may be stained with a panel of fluorescent antibodies prior to running flow.
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