I have one issue in my antibody internalization experiment. I added antibodies to incubate with cells on cell culture plate for 2-6 hr ,and then fixed/permeabilized  cells and  used secondary antibodies conjugated Alexa 488 to detect the cellular location of incubated antibodies. However, I found there is very strong fluorescence background on my plate. It seems the incubated antibodies bind on the bottom of cell culture plate.

Have anyone had the same problem? Please let me know if you have any suggestion to improve.

Thank you 

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