Hello everybody,

I want to analyze yeast cells in flow cytometry (excitation 488 nm) by use of a fluorescence indicator (GFP). I've got the problem, that autofluorescence of yeast cells is higher than the single of my fluorescence dye. So I thought about, how to minimize the autofluorescence of yeasts. Or would a plasmolysis of the cells (removal of intracellular parts) would be a solution for such problems.

Could you tell me your opinion about this topic?

Thanks in advance.

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