I am curious to know about the effects of fixation, if any, esp. by paraformaldehyde (2-4%) on cell surface markers (and also intra-cellular proteins) and subsquent flow cytometry analysis of cells, esp. of mouse bone marrow, spleenocytes, PBMCs, etc. If so, what is the correct method or timing of fixation. Is it before or after staining of cells?
@Harald, Romy and Felix: Thank you for your inputs. They are indeed helpful.
I agree with Romy Hackbusch .
I have additional suggestion,
Do not use PFA above 1%, and fixation time exceeding 10-15 minutes. Longer fixation results in increased autofluorescence.
Use 0.1 % BSA in subsequent staining or washing step to quench any PFA left behind. If there is any PFA left behind, it will non-specifically cross-link your test antibody to the cells leading to non-specific signal and background.
I hope this will solve your problem.
Let me know if you need more details.
All the best.
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