All cell populations including negative controls show elevated fluorescence, reducing signal-to-noise ratio and making it difficult to distinguish positive from negative populations.
2Two-step staining with biotinylated antibodies detecting endogenous intracellular biotin via streptavidin or anti-biotin secondary conjugates
3Dead cells with compromised membranes non-specifically binding antibodies; viability dyes incompatible with fixation protocol
4High autofluorescence in certain cell types (neutrophils) or use of autofluorescence-prone fluorochromes (FITC, Pacific Blue) instead of red-shifted alternatives
Solutions
1Use CST recommended antibody dilution (optimized for 10⁵-10⁶ cells); perform own titration when using low cell numbers
2Avoid biotinylated antibodies for intracellular staining due to endogenous biotin detection; whenever possible perform direct staining instead of two-step
3Use viability dyes compatible with fixation: fixable dyes (e.g., eFluor) for fixed cells, PI or 7-AAD for live surface staining only
4For autofluorescence-prone cells: use red-shifted fluorochromes (APC instead of FITC/Pacific Blue), or use brighter fluorochromes (Alexa Fluor 488 instead of FITC, Brilliant Violet 421 instead of Pacific Blue), or amplify signal with biotin-streptavidin/primary-secondary steps