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Flow Cytometry (Sample Considerations) moderate

Surface Epitope Masked After Fixation

Symptom
Surface marker staining fails or weakens when performed after cell fixation. Some antibody clones lose binding capacity to fixed cells.
Common Causes
  1. 1 Paraformaldehyde fixation induces protein crosslinking that masks epitopes
  2. 2 Conformational epitopes are disrupted by fixative-induced structural changes
  3. 3 Specific antibody clones are not compatible with post-fixation surface staining
  4. 4 Fixation protocol (concentration, time, temperature) not optimized for target epitope preservation
Solutions
  1. 1 Perform surface staining before cell fixation as the default workflow
  2. 2 Consult BioLegend Fixation page to identify antibody clones compatible with post-fixation surface staining
  3. 3 Contact BioLegend technical support (tech@biolegend.com) if clone compatibility information is unavailable
  4. 4 Test alternative antibody clones targeting the same marker for fixation tolerance
  5. 5 Optimize fixation conditions (e.g., 1-4% paraformaldehyde, 10-20 minutes, 4°C or room temperature) for each critical marker
  6. 6 Use fixation-compatible fluorophores and avoid tandem dyes prone to dissociation
Related Video (3)
BioLegend ★ 85
Surface and Intracellular Cytokine Staining for Flow Cytometry
"Directly addresses surface and intracellular staining with fixation step in flow cytometry, covering the exact technique where epitope masking occurs"
Bilibili (China-Accessible Mirrors) ★ 78
Flow Cytometry Complete Workflow: Sample to Analysis
"Complete flow cytometry workflow including sample preparation and staining protocols where fixation-induced epitope masking is a critical consideration"
Bilibili (China-Accessible Mirrors) ★ 72
Flow Cytometry Experimental Operation in 7 Minutes
"Hands-on flow cytometry protocol demonstration showing sample preparation and staining procedures relevant to understanding when fixation artifacts emerge"
Source: biolegend.com ↗
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