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Flow Cytometry (Fixation Buffers) severe

Low or Diminished Fluorescence Signal After Fixation

Symptom
Flow cytometry data shows weak or absent fluorescence signals from labeled antibodies following fixation step. Expected positive populations appear dim or shift toward negative, compromising detection sensitivity.
Common Causes
  1. 1 Inadequate fixation time resulting in poor antigen stabilization
  2. 2 Incorrect fixation buffer concentration (outside 1-4% paraformaldehyde range)
  3. 3 Incompatibility between specific fluorophores and chosen fixative chemistry
  4. 4 Over-fixation causing fluorophore quenching or epitope masking
  5. 5 Use of alcohol-based fixatives with sensitive fluorophores without compatibility verification
Solutions
  1. 1 Optimize fixation duration empirically for each antibody-fluorophore combination
  2. 2 Use recommended paraformaldehyde concentrations between 1-4% for protein preservation
  3. 3 Verify fluorophore-fixative compatibility before protocol implementation, especially with alcohol-based buffers
  4. 4 Avoid prolonged fixation exposure; monitor time carefully to prevent over-fixation
  5. 5 Test paraformaldehyde-based buffers as alternative when alcohol-based fixation shows fluorophore loss
Related Video (3)
BioLegend ★ 85
Surface and Intracellular Cytokine Staining for Flow Cytometry
"Directly covers fixation step in flow cytometry staining protocol, essential for understanding how inadequate fixation time causes fluorescence signal loss."
Bilibili (China-Accessible Mirrors) ★ 78
Flow Cytometry Complete Workflow: Sample to Analysis
"Complete workflow including fixation and troubleshooting section provides context for identifying and correcting inadequate fixation procedures."
Cell Signaling Technology ★ 72
Formaldehyde vs. alcohol fixation for immunofluorescence (IF) | CST Tech Tips
"Compares different fixation methods (formaldehyde vs alcohol) which directly relates to fixation quality and fluorescence signal preservation."
Source: abcam.com ↗
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