Autofluorescence Interferes with Detection Channels
Symptom
High background fluorescence observed in BV421, FITC, and PE channels, particularly with myeloid cells (monocytes, macrophages, neutrophils, eosinophils). Positive signal difficult to distinguish from cellular autofluorescence.
Common Causes
1Natural fluorescence from mitochondria, lysosomes, and NADPH emits in shorter wavelength channels (BV421, FITC, PE)
2Larger and more granular myeloid cells contain elevated levels of intracellular fluorescent compounds
3Cell size, metabolic activity, and granularity increase autofluorescence intensity
4Neutrophils and eosinophils show particularly high autofluorescence in FITC channel
Solutions
1Avoid assigning dim antigens to BV421, FITC, and PE channels when analyzing myeloid-rich samples
2Place bright markers or highly expressed antigens in autofluorescence-prone channels
3Include unstained controls for each cell subset to quantify baseline autofluorescence
4Consider using longer wavelength fluorophores (APC, AF647, AF700) for dim antigens on granular cells
5Use autofluorescence extraction algorithms during data analysis if available