No protein bands are visible on the blot, even at the expected molecular weight position. Film or imaging system shows no detectable chemiluminescence or fluorescence.
Common Causes
1Primary antibody raised against species different from sample (sequence mismatch)
2Secondary antibody incompatible with primary antibody host species or immunoglobulin class
3Primary antibody designed for native protein used on denatured Western blot samples
4HRP-labeled antibodies used in solutions containing sodium azide inhibitor
5Antibody concentration far too low to detect target protein
6Detection reagent sensitivity range does not match target protein abundance
Solutions
1Verify primary antibody targets the protein sequence from your sample species using NCBI protein database (http://www.ncbi.nlm.nih.gov/protein)
2Ensure secondary antibody targets the host species of primary antibody and matches IgG class (most common); use phylogenetically distant host from sample species
3Use antibody raised against denatured antigen for Western blot, or run non-denaturing gel for native protein antibodies
4Remove all sodium azide from buffers when using HRP-conjugated detection system