Complete lack of staining observed in immunohistochemistry experiment despite using validated antibody. Tissue sections appear negative even when positive control should show signal.
Common Causes
1Antibody not validated for IHC application or tissue type
2Sample is truly negative for the target protein (especially for phospho-specific antibodies or rarely expressed proteins)
3Slides stored improperly or for extended periods; protein epitopes degraded during storage
4Tissue sections dried out during staining procedure; sections not kept covered in liquid throughout protocol
5Inadequate deparaffinization causing spotty, uneven staining that appears as no signal
6Chemical crosslinks from fixation preventing antibody access to masked antigen targets
Solutions
1Verify antibody is validated for IHC and use high-expressing positive control (paraffin-embedded cell pellets)
2Confirm sample expression status; accept that phospho-antibodies may not stain 100% of cases
3Use freshly cut slides before experiments; if storage necessary, keep at 4°C without baking
4Ensure tissue sections remain covered in liquid throughout entire staining procedure
5Repeat experiment with new tissue sections using fresh xylene for deparaffinization
6Optimize antigen retrieval: use microwave (preferred) or pressure cooker, not water bath; prepare fresh 1X buffer solutions daily