Western blot shows no visible band for the target protein, or the band intensity is much weaker than expected, indicating little or no protein was eluted from the immunoprecipitation.
Common Causes
1Protein degradation, dephosphorylation, or denaturation during lysis due to inadequate protease/phosphatase inhibitors or incorrect temperature
2Lysis buffer stringency too high, disrupting antibody-antigen interactions
3Antibody not properly bound to beads due to isotype mismatch
4Insufficient antibody-antigen binding due to low antibody or bead concentration
5Agarose beads accidentally aspirated and removed during precipitation/wash steps
6Target protein remains bound to beads due to inadequate elution conditions (wrong buffer type or pH)
7Mouse IgG or chicken antibody used with protein G or protein A beads in indirect IP without bridging antibody
Solutions
1Perform all steps at 4°C and ensure adequate amount of protease and phosphatase inhibitors are added to lysis buffer
2Switch to medium or low-stringency lysis buffer such as NP-40-, Triton X-100-, or PBS-based buffer
3Ensure beads are properly matched to antibody isotype using the vendor affinity guide (Protein A, Protein G, A/G mix, or Kappa/Lambda binders)
4Increase antibody concentration added to lysate and/or bead concentration; extend incubation time between antibody and lysate
5Use magnetic beads instead of agarose beads to minimize/eliminate bead loss during aspiration steps
6Verify elution buffer type and pH are appropriate for the antibody-antigen complex being studied
7Add bridging antibody during precipitation step when using mouse IgG or chicken antibodies with protein G or protein A beads
8For low protein concentration or low antibody-protein affinity, switch from direct to indirect immunoprecipitation method