Target protein bands are absent or very faint on the blot, even after extended exposure times. Positive control samples may also show weak or no signal.
Common Causes
1Reusing pre-diluted antibodies: diluted antibody is less stable and prone to microbial contamination
2Insufficient protein loading: less than 20-30 µg per lane for whole cell extracts, or less than 100 µg per lane for modified targets in tissue extracts
3Low basal expression of phosphorylated or modified proteins without appropriate treatment or stimulation
4Incomplete cell lysis without sonication: membrane-bound and organelle proteins poorly extracted, nuclear DNA interferes with gel loading
5Wrong primary antibody dilution buffer: non-fat dry milk too stringent for many antibodies, reducing sensitivity
6Sub-optimal transfer conditions: standard 20% methanol transfer buffer causes poor transfer of high MW proteins (>100 kDa)
Solutions
1Always use freshly diluted antibody for each experiment; discard diluted antibody after use
2Load at least 20-30 µg protein per lane for whole cell extracts; increase to 100 µg per lane for modified targets in tissue extracts