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Anti-HA Troubleshooting

Troubleshooting for Anti-HA Antibody

Anti-HA (12CA5) recognizes the 9-amino acid sequence YPYDVPDYA derived from the human influenza hemagglutinin (HA) protein. This epitope is also recognized in fusion proteins regardless of its position (N-terminal, C-terminal or internal). The following troubleshooting information relates to immunodetection applications, such as dot blots, immunochemistry, immunoprecipitation, and Western blotting.

Anti-HA (12CA5) (Product No. ROAHA)

Chemiluminescent or chromogenic signal weak or not visible

  • Poor isolation of tagged protein
    — Use a different cell lysis procedure
  • Antibody too dilute
    — Double the concentration of the Anti-HA and/or the secondary antibody
  • Not enough protein on the gel
    — Add more protein to gel.
  • Poor transfer of proteins from gel to membrane
    — Increase the electrical current and/or the transfer time for the blot. Be sure there are no air bubbles between the membrane and gel during transfer.
  • Wrong type of membrane
    — For maximum signal, use PVDF membranes for transfer.
  • Antibody incubation too short
    — Incubate Anti-HA and/or the secondary antibody with the membrane blot for a longer time.
  • Signal development time too short
    — Double the development time.
  • Wash time too long or too stringent
    — Shorten the washing time. Omit Tween 20 from the Wash Buffer.
  • Enzyme on antibody conjugate inactivated by preservative
    — Do not use sodium azide in any Western blot reagent when using peroxidase-conjugated antibodies.
  • Substrate inactive
    — Make fresh dilution of substrate or start with a different stock of substrate.
  • Epitope tag sequence is not detectable due to proteolytic cleavage
    — Include protease inhibitors in lysis buffer.
  • Epitope tag sequence is not detectable due to low level of expression
    — Use alternative expression system or optimize your expression system. Insert multiple tag sequences into target protein to increase avidity of antibody reaction.
  • Epitope tag sequence is not detectable due to premature translation termination resulting in loss of C-terminal tag
    — Use alternative insertion site within the target gene for the epitope tag sequence.


High background additional bands on blot

  • Antibody too concentrated
    — Reduce concentration of anti-HA and/or secondary antibody by half.
  • Wash time too short
    — Prolong wash time.Incubation of membrane with substrate too long — Leave blot membrane in substrate for a shorter time.
  • Wrong type of membrane
    — For minimum background, use PVDF membranes for transfer.
  • Blocking reagent too dilute
    — Use nonfat dry milk (5% w/v) dissolved in reagent diluent as blocking reagent. Note: High concentrations of nonfat dry milk may reduce specific signal as well as background.
  • Contaminated reagents or equipment
    — Use clean equipment, freshly prepared buffers, and new membranes. Always avoid touching membranes with bare hands; use gloves and forceps.
  • Secondary antibody binds untagged proteins.
    — Use an F(ab′)2 fragment of a secondary antibody, rather than an intact IgG.
  • Heavy and light chains of primary antibody visible on blot membrane
    — Use direct detection with peroxidase-conjugated monoclonal antibody to visualize tagged proteins.
  • Signal development time too long
    — Reduce development time by half.
Materials
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