Protein bands appear faint or barely visible on the Western blot membrane or film despite proper loading. Signal intensity is insufficient for detection or quantification.
Common Causes
1Blocking reagent has affinity for target protein, masking epitopes
2Antibody concentration too low or antibody degraded by multiple freeze-thaw cycles
3Insufficient antibody incubation time
4Detection reagent outdated or HRP inhibited by sodium azide in buffer
5Using monoclonal antibody instead of polyclonal (fewer epitopes)
6Chromogenic detection substrate inactivated by tap water instead of Milli-Q water
Solutions
1Switch blocking reagent (e.g., from BSA to casein) or reduce blocking time/concentration
2Increase primary and secondary antibody concentration; prepare fresh aliquots; protect fluorescent antibodies from light
3Extend antibody incubation time (overnight at 4°C for primary antibody)
4Use fresh chemiluminescent substrate; eliminate sodium azide from all buffers
5Switch to polyclonal primary antibody for multiple epitope recognition, or use biotin-conjugated secondary antibody for signal amplification
6Prepare all chromogenic reagents with Milli-Q water; rewet dried chromogenic blots in water